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Transcript 
Foodborne antimicrobial resistance as a biological hazard1
Scientific Opinion of the Panel on Biological Hazards
(Question No EFSA-Q-2007-089)
Agreement by the BIOHAZ Panel for public consultation 5-6 March 2008
Public consultation 17 April - 27 May 2008
Adopted on 9 July 2008
PANEL MEMBERS
Olivier Andreoletti, Herbert Budka, Sava Buncic, Pierre Colin, John D. Collins, Aline De
Koeijer, John Griffin, Arie Havelaar, James Hope, Günter Klein, Hilde Kruse,
Simone Magnino, Antonio Martinez López, James McLauchlin, Christophe Nguyen-Thé,
Karsten Noeckler, Birgit Noerrung, Miguel Prieto Maradona, Terence Roberts, Ivar Vågsholm,
Emmanuel Vanopdenbosch.
SUMMARY
The European Food Safety Authority (EFSA) asked its Panel on Biological Hazards to identify,
from a public health perspective, the extent to which food serves as a source for the acquisition,
by humans, of antimicrobial-resistant (AMR) bacteria or bacteria-borne antimicrobial resistance
genes, to rank the identified risks and to identify potential control options for reducing
exposure.
The present extent of exposure to AMR bacteria was found to be difficult to determine, and the
role of food in the transfer of resistance genes insufficiently studied. Nevertheless, foodborne
bacteria, including known pathogens and commensal bacteria, display an increasing, extensive
and diverse range of resistance to antimicrobial agents of human and veterinary importance, and
any further spread of resistance among bacteria in foods is likely to have an influence on human
exposure. By way of an example, a qualitative ranking of food (ending at point of purchase) as
a vector of an AMR bacterium demonstrated the complexity of the problem and the extensive
data requirements for a formal risk ranking.
1
For citation purposes: Scientific Opinion of the Panel on Biological Hazards on a request from the European Food Safety
Authority on foodborne antimicrobial resistance as a biological hazard. The EFSA Journal (2008) 765, 1-87
© European Food Safety Authority, 2008
Foodborne Antimicrobial Resistance
In all cases where antimicrobial treatment in humans is indicated, resistance to the
antimicrobials of choice is of clinical importance. Resistant Salmonella and Campylobacter
involved in human disease are mostly spread through foods. With regards to Salmonella,
contaminated poultry meat, eggs, pork and beef are prominent in this regard. For
Campylobacter, contaminated poultry meat is prominent. Cattle are a major verotoxigenic
Escherichia coli (VTEC) reservoir and resistant strains may colonize humans via contaminated
meat of bovine origin more commonly than from other foods. Animal-derived products remain
a potential source of meticillin-resistant Staphylococcus aureus (MRSA). Food-associated
MRSA, therefore, may be an emerging problem. Food is also an important source for human
infections with antimicrobial resistant Shigella spp. and Vibrio spp.
The principles that are applied to the prevention and control of the spread of pathogenic
bacteria via food will also contribute to the prevention and the spread of antimicrobial-resistant
pathogenic bacteria. As antimicrobial resistance in foodborne pathogens and commensals
represents a specific public health hazard, additional control measures for antimicrobialresistant bacteria may therefore be necessary. There are few examples of control programmes
that directly control AMR as the hazard, using measures that specifically address food. In terms
of impact, controls operated at the pre-harvest phase, for example, those aimed at the control
and limitation of antimicrobial usage, are potentially the most effective and as such are capable
of playing a major role in reducing the occurrence of AMR bacteria in food as presented for
sale.
The development and application of new approaches to the recognition and control of food as a
vehicle for AMR bacteria and related genes based on epidemiological and source attribution
studies directed towards fresh crop-based foods, raw poultry meat raw pigmeat and raw beef are
recommended.
Specific measures to counter the current and developing resistance of known pathogenic
bacteria to fluoroquinolones as well as to 3rd and 4th generation cephalosporins found in a
variety of foods and in animals in primary production now require to be defined and put in
place as a matter of priority.
A major source of human exposure to fluoroquinolone resistance via food appears to be poultry,
whereas for cephalosporin resistance it is poultry, pork and beef that are important, these food
production systems require particular attention to prevent spread of such resistance from these
sources.
If a full risk assessment for a specific food-bacterium-combination, in respect of AMR, should
be undertaken, methodologies currently available for the risk assessment of foods require to be
modified for uniform adaptation at both MS and EU level for the risk assessment of those
combinations (including foods originating from food animals, fish, fresh produce (e.g. lettuce
etc.) and water, as a vehicle for the transmission of AMR bacteria and related genes).
Overall, control of all the routes by which AMR bacteria and their related genes can arise in the
human patient, of which food is but one such route, requires a response from all stakeholders to
acknowledge their responsibilities for preventing both the development and spread of AMR,
each in their own area of activity including medicine, veterinary medicine, primary food animal
production, food processing and food preparation, as well as in the regulation of food safety.
Key words: Antimicrobial resistance, food, Salmonella, Campylobacter, VTEC, MRSA,
Shigella, Enterococcus, Escherichia coli, Listeria monocytogenes.
The EFSA Journal (2008) 765, 2-87
Foodborne Antimicrobial Resistance
TABLE OF CONTENTS
Panel Members............................................................................................................................................1
Summary .....................................................................................................................................................1
Table of Contents ........................................................................................................................................3
Background as provided by EFSA ..............................................................................................................6
Terms of reference as provided by EFSA ...................................................................................................7
Acknowledgements .....................................................................................................................................7
Assessment..................................................................................................................................................8
1. Introduction ........................................................................................................................................8
2. Relevant antimicrobials and definition of antimicrobial resistance.................................................10
2.1.
Antimicrobials of human and veterinary importance ..............................................................10
2.2.
Definitions of resistance ..........................................................................................................11
2.2.1. Clinical resistance ...............................................................................................................11
2.2.2. Microbiological resistance ..................................................................................................11
2.2.3. Inherent (intrinsic) resistance..............................................................................................11
2.2.4. Acquired resistance .............................................................................................................12
2.2.5. Cross-resistance...................................................................................................................12
2.2.6. Co-resistance .......................................................................................................................12
2.2.7. Multiple resistance ..............................................................................................................12
3. Hazard identification ........................................................................................................................13
3.1.
Direct and indirect hazards ......................................................................................................13
3.2.
Resistance mechanisms and hazards .......................................................................................13
3.3.
Resistance transfer and hazard ................................................................................................13
3.3.1. Transfer of antimicrobial resistance to bacteria by conjugation .........................................13
3.3.2. Transfer of antimicrobial resistance by transduction..........................................................14
3.3.3. Transfer of antimicrobial resistance to bacteria by transformation ....................................14
3.4.
Food processing technologies and possible antimicrobial resistance development ................14
3.5.
Bacteria with multiple resistance as a hazard..........................................................................14
3.6.
Links between resistance and virulence as a hazard................................................................14
3.7.
The hazard of the bacterium as a carrier of resistance genes ..................................................15
3.8.
Transmission and exposure routes...........................................................................................16
4. Examples of hazards.........................................................................................................................17
4.1.
Human pathogens ....................................................................................................................17
4.1.1. Non-typhoid Salmonella......................................................................................................17
4.1.1.1. Hazard identification and characterization.................................................................17
4.1.1.2. Exposure through foods..............................................................................................18
4.1.1.3. Reports linking foodborne AMR Salmonella to human infections ............................18
4.1.2. Typhoidal Salmonella..........................................................................................................19
4.1.2.1. Hazard identification and characterisation .................................................................19
4.1.2.2. Exposure through foods..............................................................................................19
4.1.2.3. Reports linking foodborne AMR Salmonella Typhi to human infections..................20
4.1.3. Thermophilic Campylobacter..............................................................................................20
4.1.3.1. Hazard identification and characterization.................................................................20
4.1.3.2. Exposure through foods..............................................................................................21
4.1.3.3. Reports linking foodborne AMR Campylobacter to human infections .....................22
4.1.4. Verotoxigenic Escherichia coli (VTEC) of public health concern .....................................22
4.1.4.1. Hazard identification and characterization.................................................................22
4.1.4.2. Exposure through foods..............................................................................................23
4.1.4.3. Reports linking foodborne AMR VTEC to human infections....................................23
4.1.5. Shigella................................................................................................................................24
4.1.5.1. Hazard identification and characterization.................................................................24
4.1.5.2. Exposure through foods..............................................................................................24
The EFSA Journal (2008) 765, 3-87
Foodborne Antimicrobial Resistance
4.1.5.3. Reports linking foodborne AMR Shigella to human infections .................................24
4.1.6. Vibrio ..................................................................................................................................25
4.1.6.1. Hazard identification and characterization.................................................................25
4.1.6.2. Exposure through foods..............................................................................................25
4.1.6.3. Reports linking foodborne AMR Vibrio spp. to human infections ............................25
4.1.7. Meticillin-resistant Staphylococcus aureus (MRSA)..........................................................25
4.1.7.1. Hazard identification and characterisation .................................................................26
4.1.7.2. Exposure through foods..............................................................................................27
4.1.7.3. Reports linking foodborne MRSA to human infections.............................................27
4.1.8. Listeria monocytogenes.......................................................................................................27
4.1.8.1. Hazard identification and characterisation .................................................................27
4.1.8.2. Exposure through foods..............................................................................................28
4.1.8.3. Reports linking foodborne AMR L. monocytogenes to human infection...................28
4.2.
Commensals.............................................................................................................................28
4.2.1. Escherichia coli ...................................................................................................................28
4.2.1.1. Hazard identification and characterisation .................................................................28
4.2.1.2. Exposure through foods..............................................................................................29
4.2.1.3. Reports linking foodborne AMR E. coli to human infections....................................29
4.2.2. Enterococcus .......................................................................................................................29
4.2.2.1. Hazard identification and characterization.................................................................30
4.2.2.2. Exposure through foods..............................................................................................30
4.2.2.3. Reports linking foodborne AMR enterococci to human infections............................30
4.3.
Bacteria deliberately added to the food chain or being an integral part of the food ...............31
4.3.1. Hazard identification and characterisation..........................................................................31
4.3.2. Exposure through foods.......................................................................................................32
4.3.3. Antimicrobial-resistant starter and probiotic bacteria and human infections .....................32
5. Categorisation of food with respect to risk of AMR........................................................................33
5.1.
Source attribution ....................................................................................................................34
6. On assessing the risk of the acquisition of antimicrobial resistant bacteria or bacteria-borne
antimicrobial resistance genes via the food chain.....................................................................................36
6.1.
Issues to be considered in relation to risk assessment applied to the area of antimicrobial
resistance...............................................................................................................................................36
6.1.1. Data requirements for an antimicrobial resistance risk assessment ....................................37
6.1.2. Requirements for a risk assessment....................................................................................39
6.2.
Construction of an exposure assessment template: Food as a source of antimicrobial resistant
bacteria. An example. ...........................................................................................................................40
6.2.1. Exposure pathway ...............................................................................................................40
6.2.2. Data requirements and availability......................................................................................41
6.2.2.1. Probability of bacteria being present in food at retail ................................................42
6.2.2.2. Probability that bacteria present in food at retail are resistant to antimicrobial class
of interest 42
6.2.2.3. Probability of AMR bacteria in food at retail.............................................................42
6.2.2.4. Probability that food is purchased and prepared for consumption .............................42
6.2.3. Presenting the risk estimate.................................................................................................42
6.2.4. Case-study 1: Fluoroquinolone-resistant Campylobacter jejuni in the UK ........................42
6.2.5. Future development of risk assessment approaches............................................................44
6.2.6. Antimicrobial resistance genes in genetically modified organisms ....................................45
7. Prevention and control options.........................................................................................................46
7.1.
Controlling spread of infections and of resistant bacteria.......................................................47
7.1.1. Preventing infectious diseases in animals and plants..........................................................47
7.1.2. Control and prevention of Salmonella and other zoonotic bacteria in animals ..................47
7.1.3. Improved hygiene ................................................................................................................47
7.1.4. Processing............................................................................................................................47
7.1.5. Recirculation .......................................................................................................................47
The EFSA Journal (2008) 765, 4-87
Foodborne Antimicrobial Resistance
7.2.
Appropriate usage of antimicrobials........................................................................................48
8. Issues of immediate concern ............................................................................................................48
Conclusions and Recommendations .........................................................................................................49
Appendices................................................................................................................................................72
The EFSA Journal (2008) 765, 5-87
Foodborne Antimicrobial Resistance
BACKGROUND AS PROVIDED BY EFSA
Antimicrobial resistant bacteria are biological hazards2 associated with increased human
morbidity and mortality and are of public health concern. The use of antimicrobial agents in
animals, plant production and the production of other sources of food and feed has adverse
public health consequences by creating a reservoir of resistant bacteria and of bacteria-borne
resistance genes that can be passed on to humans, both directly or indirectly. Such resistance
respects neither phylogenetical, geographical nor ecological borders. Mobile genetic elements
harbouring resistance determinants can readily be transferred horizontally between bacteria
from terrestrial animals, fish and humans; furthermore, such transfer can take place in natural
environments such as the kitchen.
The use of antimicrobial agents for the treatment and control of infectious diseases in animals
and crops continues because of considerations regarding animal health and welfare, and plant
health. Consequently the transfer of antimicrobial-resistant bacteria and bacteria-borne
resistance genes from animals or crops to humans via food remains a matter of public health
concern.
The use of antimicrobials at subtherapeutic levels in food producing animals has long been
viewed as undesirable e.g. the Swann report, 19693. Since January 2006 the use of all
antimicrobial feed additives has been banned within the EU in order to reduce the numbers of
resistant bacteria in farm animals (Regulation (EC) No 1831/2003 of the European Parliament
and of the Council of 22 September 2003 on additives for use in animal nutrition)4. The effect
of this ban on the extent of bacterial antimicrobial resistance both within farm animals, and
with regard to human health, however, is unclear.
Use of antimicrobial agents is the main driver for the development and spread of antimicrobial
resistance. In addition, spontaneous mutation in foodborne bacteria or the spread of resistant
bacteria in the absence of selective pressure may also contribute to the antimicrobial resistance
burden in food.
Antimicrobial-resistant bacteria and bacteria-borne resistance genes can be spread to humans
via food by different routes and mechanisms, for example:
•
By foodborne spread of resistant zoonotic bacteria, e.g. Salmonella and Campylobacter.
These bacteria may originate from various sources, including animals, the environment and
humans.
•
By foodborne spread of resistant non-zoonotic human pathogenic bacteria e.g. Shigella spp.
and Vibrio spp. These bacteria do not have a primary reservoir in food animals, but can be
spread from humans to food directly or indirectly through the environment, including water.
•
By foodborne spread of resistant commensal bacteria carrying transferable antimicrobial
resistance genes that can be passed on to human pathogenic bacteria. These resistant
commensal bacteria may originate from various sources, including animals, the
environment and humans.
2
Hazard- “a biological, chemical or physical agent in, or condition of, food with the potential to cause an adverse health
effect”
3
Swann MM. Report of the Joint Committee on the use of antibiotics in animal husbandry and veterinary medicine. London:
Her Majesty’s Stationary Office; 1969.
4
More precisely: Since January 2006 the use of antibiotics other than coccidiostats and histomonostats as feed additives has
been banned within the EU (Regulation (EC) No 1831/2003 of the European Parliament and of the Council of 22
September 2003 on additives for use in animal nutrition)
The EFSA Journal (2008) 765, 6-87
Foodborne Antimicrobial Resistance
The foodborne route of transfer of antimicrobial resistance is in addition to direct zoonotic
spread resulting from contact with animals, e.g. livestock, pets and their excreta. Meanwhile,
foods other than those originating from animals can also be vectors for the transmission of
antimicrobial-resistant bacteria and bacteria-borne resistance genes to the consumer. In
addition, food handlers can contaminate food during preparation, as has happened, for example,
in the case of both meticillin-resistant Staphylococcus aureus (MRSA) and resistant Shigella
spp. Finally, as already mentioned, the presence of antimicrobial-resistant bacteria in food may
be the result of environmental contamination, e.g. from water sources, in the case of
aquacultural and horticultural produce in particular. The extent and relative importance of the
contribution of each of these pathways to the risk of antimicrobial resistance in microorganisms
of human health concern is unknown.
On 17 April 2008, EFSA published the draft opinion of the BIOHAZ Panel on the self-tasking
mandate on foodborne antimicrobial resistance as a biological hazard and invited comments.
The closure date of the consultation was 27 May 2008.
Twelve submissions of public comments were received from individuals, food processors,
member states food safety authorities, European Community agencies and associations
representing sectors of the European food industry. EFSA and the Panel on Biological Hazards
(BIOHAZ) wish to acknowledge and thank those who provided comments. EFSA and the
BIOHAZ Panel took into consideration all the received comments and, where appropriate,
modified the draft opinion.
TERMS OF REFERENCE AS PROVIDED BY EFSA
The Scientific Panel on Biological Hazards is asked, from a public health perspective,
1. To identify in terms of qualitative risk5, the extent to which food serves as a source for
the acquisition, by humans of antimicrobial-resistant bacteria or bacteria-borne
antimicrobial resistance genes.
2. To rank the identified risks.
3. To identify potential control options for reducing exposure.
ACKNOWLEDGEMENTS
The European Food Safety Authority wishes to thank the members of the Working Group for
the preparation of this opinion: Frank Aarestrup, Patrick Butaye, John D. Collins (Chair),
Seamus Fanning, Christina Greko, Arie Havelaar, Lieve Herman, Günter Klein (Rapporteur),
Antonio Martinez López, Emma Snary, Eric John Threlfall, Atte von Wright. Assistance to the
Working Group from James McLauchlin is also acknowledged.
5
Risk is defined as “a function of the probability of an adverse health effect and the severity of that effect, consequential to a
hazard(s) in food”, Codex Alimentarius Commission, Procedural Manual.
The EFSA Journal (2008) 765, 7-87
Foodborne Antimicrobial Resistance
ASSESSMENT
1.
Introduction
Many scientific reviews have focussed on antimicrobial resistance in zoonotic bacterial
pathogens and the possible link between the use of veterinary antimicrobials, prophylactics and
growth promoters and resistance issues in human medicine (ACMSF, 1999; Anderson, 2003). If
strategic prevention and controls are to be effective, it is important to better understand the
ecology, epidemiology and extent of such resistance among food-borne pathogens.
The consequences of the use of antimicrobials6 in primary animal production and to a lesser
extent in other areas of food production including aquaculture and horticulture have been
reviewed elsewhere. Notwithstanding this, to date the contribution of food in all its processed
and non-processed forms has not been studied in detail. In particular, the relative contribution
of food to the occurrence of antimicrobial resistance to critically important antimicrobials in
bacteria causing disease in humans has not been the subject of scientific opinions. In this
Opinion the ways in which food serves as a vehicle for the acquisition of antimicrobial-resistant
bacteria or bacteria-borne antimicrobial resistance genes causing infections in humans is
addressed with a view to conducting an initial ranking of the identified risks and identifying
potential control options.
The issue of antimicrobial resistance (AMR) is of world wide concern. The ECDC in its
review of 2005 data on communicable diseases in Europe, identified AMR as a major problem
in European health care, and one that undoubtedly prolongs patient suffering, costs money and
is responsible for the death of thousands of European citizens each year (ECDC, 2007). The
WHO, FAO, including Codex, and OIE have each (individually or jointly) reviewed the area
and provided guidelines, recommendations and lists of clinically important antimicrobials (e.g.
FAO/OIE/WHO, 2003; WHO, 2007). The latest activity in this area is the Codex Ad Hoc
Intergovernmental Task Force on Antibiotic Resistance (Codex, 2007), which aims to assess
the risks to human health associated with the presence in food and feed of antimicrobialresistant organisms, and genes, and to develop risk management advice based on that
assessment to reduce such a risk.
The most important factor influencing the emergence and spread of AMR is the use of
antimicrobial agents in different hosts with spread of resistant bacteria and resistance genes
between hosts of the same or of different species (SSC, 1999). In the human, veterinary and
horticultural spheres there is a variety of ways in which antimicrobials come to be dispensed
and applied. In human medicine, antimicrobials are widely used for therapy and prophylaxis
both in hospitals and in the community, under varying levels of supervision. Likewise, as
already mentioned in the Background to this Opinion, the same antimicrobial agents continue to
be widely used in animals and aquatic species bred for food production, for therapeutic
treatment, prophylaxis and growth promotion (no-longer in the EU), and also in companion
animals, for therapy and prophylaxis, also under varying degrees of supervision. Oral
medication of large groups of animals is particularly likely to favour emergence of and selection
for AMR. Also, in primary production, conditions exist that facilitate the spread of bacteria,
such as high density and/or poor infection control.
6
Antimicrobial: A drug, not a disinfectant, which, at low concentrations, exerts an action against microbial pathogens and
exhibits selective toxicity towards them (EFSA, 2004a)
The EFSA Journal (2008) 765, 8-87
Foodborne Antimicrobial Resistance
Whilst of relevance to the development of antimicrobial resistance in the microflora of humans,
consideration of the effects of residues of antimicrobial substances in food are not within the
scope of this Opinion. The development of and selection for resistance, as well as links between
resistance to biocides7 and antimicrobials (Gilbert and McBain, 2003), are briefly discussed; as
these issues are the subject of study elsewhere they are outside the terms of reference of this
mandate. Decontamination of fresh poultry carcasses with decontamination substances are dealt
with in other opinions of the respective panels of EFSA, including a specific mandate on related
antimicrobial issues (EFSA, 2006, 2008a).
Figure 1 illustrates ways in which AMR can arise in food as consumed, against a background
that includes the continued use of antimicrobials in human medicine and in food production
(see, for example, Aarestrup (2006) for other pathways of transmission of AMR bacteria to
humans). Because of their complexity, the factors that can lead to the contamination of food in
the final stages of its preparation, as in the kitchen, are not addressed in detail here. The direct
relevance of the application of good hygienic practices in this and other phases of the food
chain in preventing and controlling such contamination is emphasised.
Antimicrobial use in food production
Antimicrobial use in human medicine
Other- processed food*
Fully-processed food
packaging
packaging
Raw Food
Food from
primary
production ;
Handling
Packaging
Storage/
transport
Retail---------------------- Kitchen
sale
water
uncooked
cooked
in-kitchen contamination
pre- and/or post-cooking
Figure 1.
A schema for the possible transmission of antimicrobial resistance via food8.
Transfer of antimicrobial resistance can involve different kinds of microorganisms. Human
bacterial pathogens can be acquired directly by person-to-person spread and from the
environment, as well as from animals including both food producing animals and domestic
7
Biocides: “Active substances and preparations containing one or more active substances, put up in the form in which they
are supplied to the user, intended to destroy, deter, render harmless, prevent the action of, or otherwise exert a controlling
effect on any harmful organism by chemical or biological means." Directive 98/8/EC
8
Food from primary production includes fresh meat, fruit and vegetables. Water is also included in this category
The EFSA Journal (2008) 765, 9-87
Foodborne Antimicrobial Resistance
pets, or as foodborne pathogens directly from food. Commensal bacteria, i.e. those bacteria
belonging physiologically to the human or animal microflora and which are not primarily
considered as pathogenic for their host, can likewise be acquired by the consumer through
contaminated food or from the environment. Bacteria deliberately introduced into the food
chain for manufacturing purposes, e.g. fermentation cultures, and probiotics, likewise require to
be considered in the context of antimicrobial resistance transfer through the agency of food. In a
wider sense also, bacteria belonging to the natural food microflora belong to the latter group of
microorganisms.
In accordance with Directive 2003/99/EC, EFSA is responsible for preparing the Community
Summary Report on Trends and Sources of Zoonoses, Zoonotic Agents, Antimicrobial
Resistance and Foodborne Outbreaks in the EU. Further to this, EFSA’s Task Force on
Zoonoses Data Collection has also published proposals for harmonised monitoring schemes for
antimicrobial resistance in Salmonella in fowl (Gallus gallus), turkeys and pigs and
Campylobacter jejuni and C. coli in broilers (EFSA, 2007a), and has proposed technical
specifications for a planned baseline survey on MRSA in breeding pigs (EFSA, 2007b).
Proposed harmonisation for monitoring of antimicrobial resistance in other bacteria is under
consideration.
2.
Relevant antimicrobials and definition of antimicrobial resistance
Antimicrobials encompass antibacterial, antiviral, antifungal and antiparasitic agents. In this
document, the term will be limited to antibacterial agents classically used for therapy,
prophylaxis or until recently (in the EU), growth promotion. As explained above, the effect of
disinfectants and other biocides on antimicrobial resistance are not addressed in this document.
Antimicrobial susceptibility or resistance is generally defined on the basis of in vitro
parameters. The terms reflect the capacity of bacteria to survive exposure to a defined
concentration of an antimicrobial agent, but different definitions are used depending on whether
the objective of the investigation is clinical diagnostics (see 2.2.1) or epidemiological
surveillance (see 2.2.2).
2.1.
Antimicrobials of human and veterinary importance
Antimicrobials are grouped into classes on the basis of chemical structure and mode of action.
Most antimicrobials used for the treatment of animals belong to classes that are also used in
human medicine. A list of antimicrobial classes, examples of substances used for the treatment
of infections in humans and animals, along with comments on cross-resistance within and
between classes and examples of resistance genes described to date, are presented in Table A
(see Appendix).
The consequences of antimicrobial resistance depend on the role of the antimicrobial class in
the treatment of human disease. The World Health Organisation (WHO) convened two expert
meetings (WHO, 2005b, 2007) in order to classify antimicrobial drugs as “critically important”,
“highly important”, and “important” based on two criteria, namely (i) sole therapies or one of
few alternatives to treat serious human disease, and (ii) used to treat diseases caused by
microorganisms that may be transmitted via non-human sources or diseases caused by
microorganisms that may acquire resistance genes from non-human sources. A number of
antimicrobial classes were categorised as critically important to human health. Participants
concluded that from a public health perspective, the antimicrobial classes of greatest priority for
risk management are: quinolones, 3rd/4th generation cephalosporins and macrolides (WHO,
2007).
The EFSA Journal (2008) 765, 10-87
Foodborne Antimicrobial Resistance
Similarly, the World Animal Health Organisation (OIE) has developed and adopted a list
ranking the importance of different antimicrobials for animal health (OIE, 2007b).
2.2.
Definitions of resistance
2.2.1.
Clinical resistance
Clinically-resistant infections are defined as those infections having a low probability of
clinically responding to treatment, even if maximum doses of a given antimicrobial are
administered (EUCAST, 2000; Acar and Röstel, 2003). The outcome of a treatment depends on
many factors e.g. the pharmacokinetics of the drug, site of infection, status of the patient and
properties of the causative agent. Clinical resistance cannot, therefore, be predicted by in vitro
tests alone. The Minimum Inhibitory Concentration (MIC) of a drug for a bacterium isolated
from clinical samples is used for guidance purposes, however.
A bacterial isolate is categorized as resistant when the obtained MIC of the drug is associated
with a high likelihood of therapeutic failure of treatment with that drug. To facilitate the
interpretation, threshold values or breakpoints are defined by national or international
committees on the basis of, for example, pharmacokinetics, clinical trials and microbiology.
Clinical breakpoints are intended for use in everyday clinical laboratory work to advise on
therapy in the patient and may vary between countries and over time (Kahlmeter et al., 2003).
The fact that the clinical break-points are defined differently by a number of National
Committees hampers comparison of published data. Within EUCAST, activities to harmonise
clinical breakpoints are ongoing (Kahlmeter et al., 2003; 2006).
2.2.2.
Microbiological resistance
When a bacterium can tolerate higher concentrations of an antimicrobial than phenotypically
related bacteria of the original or “wild type” strain (Acar and Röstel, 2003), it is defined as
being resistant. Such isolates are phenotypically different from the wild type because of their
acquisition of a resistance mechanism either by gene transfer or mutation (acquired resistance).
Interpretation criteria for in vitro tests are based on the distribution of MICs among large
collections of wild-type bacteria. An isolate is categorized as resistant when the MIC of a
certain drug is higher than that which is expected for wild-type strains. An isolate classified as
resistant by this criterion may well be classified as susceptible by clinical criteria.
The values used for categorisation are termed “epidemiological cut-off values”. As they are
based on properties of a bacterial species, these interpretation criteria will not change over time
or between countries (Kahlmeter et al., 2003). The use of epidemiological cut-off values
provides an appropriate level of sensitivity when measuring resistance development in bacteria.
These criteria have been harmonised between MS and are independent of the source of the
bacterium investigated. EUCAST and EFSA have proposed the use of such criteria for
monitoring of resistance in bacteria of concern both to human and veterinary medicine in the
European Union (Kahlmeter et al., 2003; EFSA, 2006a).
In this Opinion, resistance is understood as microbiological resistance unless otherwise stated.
2.2.3.
Inherent (intrinsic) resistance
Intrinsic resistance is a trait of a bacterial species. For example, the target of the antimicrobial
agent may be absent in that species, the cell wall may have poor permeability for certain types
of molecules or the bacterial species may inherently produce enzymes that destroy the
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antimicrobial agent. These bacteria are clinically resistant, but should more accurately be
referred to as “insensitive”.
2.2.4.
Acquired resistance
A bacterial strain can acquire resistance either by mutation or by the uptake of exogenous genes
by horizontal transfer from other bacterial strains. Genes encoding enzymes that can modify the
structure of an antimicrobial are commonly transferable (penicillinases and cephalosporinases
(bla-genes), acetyl transferases modifying e.g. aminoglycosides (aac-genes), as are genes
leading to target modification (erm-genes), meticillin9-resistance (mecA-genes) and
glycopeptide-resistance (van-genes). There are several mechanisms for horizontal gene transfer,
and they often function in concert. Large plasmids with many different genes can be transferred
from bacterium to bacterium by conjugation. Transposons can carry several resistance genes.
They cannot replicate by themselves, but can move within the genome, e.g. from plasmid to
plasmid or from chromosome to plasmid. Integrons can also encode several resistance genes.
They cannot move by themselves, but encode mechanisms both to capture new genes and to
excise and move cassettes with genes within and from the integron.
2.2.5.
Cross-resistance
Antimicrobials are a diverse group of molecules, commonly ordered in classes with similar
structure and mode of action (Table A, Appendix). Within a class, the target in the bacterial cell
and the mode of action of the antimicrobial is the same or similar in each case. Therefore, some
mechanisms of resistance will confer resistance to most or all members of a class, i.e. crossresistance. Cross-resistance may also occur in relation to unrelated classes, if the target overlaps
(as in the case of macrolides and lincosamides) or if the mechanism of resistance is of low
specificity (e.g. affecting efflux pumps).
2.2.6.
Co-resistance
Genes conferring antimicrobial resistance are frequently contained in larger genetic elements
such as integrons, transposons or plasmids, and as such may be ‘linked’ to other, unrelated
resistance genes. In such cases, multiple resistance genes may be transferred in a single event.
When two or more different resistance genes are physically linked, this is termed “coresistance”. Consequently, selection for one resistance will also select for the other resistance
gene(s).
2.2.7.
Multiple resistance
Multiple resistance (MR), sometimes referred to as “multi-resistance” is used here when a
bacterial strain is resistant to several different antimicrobials or antimicrobial classes. There is
no standard definition, which makes the term problematic and comparisons difficult.
9
Meticillin (International Nonproprietry Name) = Methicillin (United States Adopted Name)
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3.
Hazard identification
3.1.
Direct and indirect hazards
The issue of antimicrobial resistance in food is addressed as existing either as a direct hazard or
as an indirect hazard through resistance transfer10. The direct hazard is the presence on food of
an antimicrobial-resistant pathogenic bacterium which can colonise or infect a human being
after ingestion of the food, or as a hazard that arises if a person acquires the infection through
handling contaminated food. The indirect hazard arises through resistance transfer and is
defined as an antimicrobial-resistant bacterium that may transfer resistance genes to a bacterium
pathogenic for humans, either directly, or via another commensal bacterium. In this case, the
hazard is considered as being the resistance gene.
3.2.
Resistance mechanisms and hazards
The resistance mechanisms involved may be classified in four large groups, as follows: (1)
Enzymatic inactivation/degradation mechanisms such as ß-lactamases degrading penicillins and
cephalosporins and aminoglycoside modifying genes. (2) Alternative pathways, such as
resistance to dihydrofolates antimicrobials e.g. sulphonamides and trimethoprim resistance. (3)
Permeability changes, rendering the bacterium impermeable (altered porins) or a change in the
rate of pumping out the antimicrobial (efflux). An example is tetracycline resistance. (4) Target
alteration such as resistance to macrolides and (fluoro)quinolone antimicrobials.
3.3.
Resistance transfer and hazard
Transfer of resistance genes between bacteria can occur at any point along the food chain, or
within one body system (e.g. the intestine), or can occur between systems (e.g. from the
intestinal tract to bacteria on the skin). These transfers can happen through three different
mechanisms, (1) Conjugation, where a mobile genetic element (plasmid, transposon, gene
cassette) can be transferred from one bacterium to another bacterium. (2) Transduction, where a
bacteriophage takes up a resistance gene from one bacterium and transfers this to another
bacterium. (3)Transformation, where naked DNA released from one bacterium is taken up by
another bacterium.
3.3.1.
Transfer of antimicrobial resistance to bacteria by conjugation
Conjugation is the mechanism by which genetic material transfers from one bacterium to
another through a protein tunnel that temporarily connects the two bacteria. Such transfer may
occur between bacteria of different species or even different genera. The elements transferred
may be plasmid- or transposon-mediated. The transposable elements may be able to induce
conjugation by themselves (self-transposable elements) or may need some functions coded by
other genetic elements belonging to the bacterium itself, or to another mobile element. This is
the most frequently reported mechanism of resistance transfer to date. The elements that are
able to transfer often contain more than one gene for resistance and may encode linked
resistance genes. One transfer may likewise deliver multiple resistances to the recipient
bacterium.
10
A bacterium may also present both a direct and indirect hazard: e.g. a resistant pathogenic bacterium with a resistance
gene(s) carried on a potentially transferable element.
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3.3.2.
Transfer of antimicrobial resistance by transduction
Transduction is the mechanism by which bacteriophages transfer genes from one bacterium to
another. By taking up host DNA from one bacterium, and after lysis of the host cell (and release
of the phages) the phage can introduce new genetic material into another (same) phagesusceptible bacterium.
3.3.3.
Transfer of antimicrobial resistance to bacteria by transformation
While the processes of conjugation and transduction require viable donor cells, this is not the
case for transformation. Successful transformation and expression of antibacterial resistance in
bacterial cells is based on the following essential steps: 1) release of the DNA from the donor;
2) uptake of the DNA by competent bacteria in the vicinity; 3) stable incorporation of the DNA
in the recipient cell and 4) expression of the incorporated DNA.
3.4.
Food processing technologies and possible antimicrobial resistance development
Most food processing technologies aim to reduce the numbers of foodborne pathogens present,
including AMR bacteria, as well as the overall bacterial load. Hence, food deterioration and the
possibility of foodborne infections are reduced. This important beneficial effect has to be
considered when evaluating any potential hazards arising from food processing with respect to
antimicrobial resistance.
Emerging non-thermal processing/preservation technologies (e.g. high-pressure processing,
ionizing radiation, pulsed electric field and ultraviolet radiation) are technologies designed to
produce safe food, while maintaining its nutritional and sensory qualities. Experimental studies
have shown that through damage to cell membranes, enzymes or DNA (Lado and Yousef
2002), such alternative preservation technologies could promote the generation or transfer of
antimicrobial resistance (Zenz et al., 1998; Davison, 1999; IFT, 2002; Lado and Yousef 2002;
Kharazmi et al., 2002; Cérémonie et al., 2004, 2006; Rodrigo et al., 2005, 2007; McMahon et
al., 2007). Whilst these studies remain at the laboratory level, the relevance for industrial food
processing remains to be defined.
3.5.
Bacteria with multiple resistance as a hazard
For many bacteria, multiple resistance may create health problems, since the use of one
antimicrobial will also select for resistance to other unrelated antimicrobials. Specific structures
(integrons) that can collect and express antimicrobial resistance genes are present in bacteria.
Furthermore, the genes encoding resistance in bacteria exhibiting multiple resistance may also
be located on separate mobile elements.
Bacteria resistant to the latest categories of antimicrobials are also more likely to be multiply
resistant (e.g. to 3rd and 4th generation cephalosporins), rendering the disease they cause more
difficult to treat and prone to therapy failure.
3.6.
Links between resistance and virulence as a hazard
Increased frequency of treatment failures and increased severity of infection due to infections
with AMR bacteria are the principal human health concerns. They may be manifested by
prolonged duration of illness, increased frequency of bloodstream infections, increased
hospitalization, or increased mortality (WHO, 2005a).
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Virulence of a bacterium is in general encoded by either a number of single genes or a cluster of
genes, interplaying at different levels of the pathogenesis. Some genes, when deleted may be so
essential in certain steps of the pathogenesis that virulence is abolished completely, while other
genes are only of additional value to the virulence of the bacterium. Frequently, virulence genes
are encoded on mobile genetic elements. Other elements contributing to pathogenicity are the
so-called ‘Pathogenicity Islands’, 12 of which have been identified in Salmonella enterica
(Hensel, 2004). Further virulence factors in some Salmonella serotypes and phage types are
those which are involved in the iron sequestration system, thereby providing their host strains
with the ability to survive in environments where iron is not readily accessible to the bacterium,
such as blood. These virulence factors can have a substantive impact on the invasive ability of
their host strains. Finally, genomic islands, such as SGI1 in S. enterica, may carry both
virulence and antimicrobial resistance genes (Golding et al., 2007). As co-localisation of
virulence genes and resistance genes on the same mobile genetic element has been reported
(Carlson et al., 2007), the transfer of resistance, and simultaneously the transfer of the coresident virulence genes, may give the bacterium, in addition to a newly acquired resistance, an
enhanced virulence.
Genes that have functions both in virulence and antimicrobial resistance are also known. An
example of this are some efflux pumps in Campylobacter (Lin et al., 2007; Quinn et al., 2007;
Piddock et al., 2006).
MRSA frequently contain the genes associated with enterotoxins (Fey et al., 2003; Yarwood et
al., 2002), which are the proteins which cause staphylococcal food poisoning. Different
combinations of enterotoxins are associated with different MRSA clones (Ferry et al., 2006;
Tristan et al., 2007). Enterotoxin genes are either located on mobile genetic elements, or within
pathogenicity islands. Increased prevalence of MRSA amongst S. aureus strains could lead to a
higher prevalence of toxinogenic S. aureus. It is not clear why there is an association with
specific lineages of MRSA and enterotoxin genes. Food poisoning due to MRSA remains very
rare (see Section 4.1.7.3).
3.7.
The hazard of the bacterium as a carrier of resistance genes
The antimicrobial-resistant bacteria that pose a particular hazard are primarily those with
resistance to the first-line drug of choice used in the treatment of a specific bacterial disease.
Central to this is that upon ingestion of, or other contact with, these bacteria, the resistance
gene(s) can be transferred directly or via an intermediary, to a human pathogenic bacterium.
The likelihood of such transfer will be higher if the host is simultaneously exposed to an
antimicrobial to which the bacteria are resistant (McConnell et al., 1991; Doucet-Populaire et
al., 1991). Furthermore, such use will amplify resistance by selecting for any resulting
transconjugants.
We can identify three different groups of resistant micro-organisms that may be of importance;
Firstly, zoonotic agents and other food borne pathogens. They can directly pose a hazard, since
in some cases, the conditions they cause need clinical treatment and, if resistant, they cannot be
successfully treated with the antimicrobials against which the bacterium is resistant. Also, some
of the bacteria remain for a certain period in the intestinal tract, where they may exchange or
acquire resistance genes.
Secondly, commensals are also a potential AMR hazard. This is largely dependent on the
capacity of the ingested food-derived commensals to come in contact with human commensals
and pathogens. As the gastro-intestinal tract is the place with the highest abundance of host
bacteria, the ability of the commensal to remain in this environment is of major importance for
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Foodborne Antimicrobial Resistance
the exchange of resistance genes. Other factors of influence are the mobile element on which
the resistance genes are located, and the ability to form biofilms.
Thirdly, “industrial” or “technological” and /or other bacteria intentionally added to the food
chain, may also be regarded as a potential hazard. These bacteria have a function in e.g.
fermentation or preservation of the food product, or may be added specifically with a health
claim, as in the case of probiotics. Bacteria added to the food chain should not carry potentially
transferable resistance genes, (FAO/WHO, 2001; EFSA, 2005a; EFSA, 2007c) as it cannot be
excluded that they may transfer their resistance genes directly or indirectly to pathogenic
bacteria.
There is a paucity of information about the total presence, nature and evolution of antimicrobial
resistance in the intestine. Likewise, there is only limited information about the rates of transfer
of antimicrobial resistance in the gastrointestinal tract involving species other than E. coli and
enterococci. Although only few data exist, mainly from in vitro models and from experiments
on mice (e.g. Doucet-Populaire et al., 1991; McConnell et al., 1991), transfer of resistance from
an ingested strain of Escherichia coli K12 to intestinal E. coli bacteria has been demonstrated in
volunteers, albeit at low frequency (Anderson 1975). Also, in vivo transfer of vanA genes from
Enterococcus faecium isolated from chicken to intestinal enterococci in human volunteers has
been detected (Lester et al., 2006).
As for resistance genes in genetically modified food products, the reader is referred to Section
6.2.6 in this document, and to EFSA (2004b).
3.8.
Transmission and exposure routes
Cross-contamination with AMR bacteria resulting from improper handling of food is a well
known phenomenon and has been widely studied (Kusumaningrum et al., 2004; Mylius et al.,
2007). Campylobacter spp. are more likely to be spread from primarily contaminated food like
fresh chicken to other food prepared in the kitchen (e.g. ready-to-eat fresh salad) than are
Salmonella spp. (Kusumaningrum et al., 2004). Fresh chicken with a high contamination level
of antimicrobial-resistant Campylobacter will be a likely source of contamination for other
foods if appropriate standards of food hygiene are not consistently applied at the distribution
and retail phases of the food chain and, in particular, in the kitchen in the course of final food
preparation and presentation.
In addition to the transmission routes mentioned above, other sources of food contamination
with AMR bacteria are the smaller companion animals such as those kept as domestic pets in
the private household.
Bacteria known to be spread by pets (such as dogs, cats, and exotic species including reptiles)
include Campylobacter, Salmonella spp. (Marcus, 2008) and MRSA (Weese et al., 2006). As
bacteria present in the intestinal tract of pets can also carry antimicrobial resistance of clinical
relevance (Rossi et al., 2007), household pets could be a direct source of AMR bacteria in the
kitchen.
Furthermore, cross-contamination in the kitchen can also result from a variety of sources
including storage facilities such as refrigerators, and the use of work surfaces and towels that
remain contaminated following the preparation of other foods (Kruse and Sorum, 1994).
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4.
Examples of hazards
4.1.
Human pathogens
4.1.1.
Non-typhoid Salmonella
4.1.1.1. Hazard identification and characterization
Salmonella is a zoonotic agent that readily infects humans. In general, treatment with
antimicrobial drugs is not recommended for cases of salmonellosis in otherwise healthy
individuals. Nevertheless, in the elderly, very young, or immunocompromised patients,
treatment with an appropriate antimicrobial can be life-saving. Likewise, should a strain spread
from the intestine to normally sterile body sites, then treatment with an appropriate drug is
essential. In such cases, infection with an antimicrobial resistant Salmonella may pose an
additional public health risk to that posed by infections that are susceptible.
Food is regarded as an important infection route for Salmonella including AMR Salmonella.
There are numerous reports directly implicating foodborne AMR Salmonella in human disease
(see 4.1.1.2 below), and a limited number of reports confirming transmission of AMR strains
from the food animal, into foods, and subsequently to the human population. In 1984, a strain
of Salmonella Newport with resistance to ampicillin and tetracyclines originating in cattle in the
USA was traced through the food chain to humans (Holmerg et al., 1984); in 1998, an outbreak
of multiresistant S. Typhimurium with additional resistance to quinolone antimicrobials, in
which 15 persons were affected was traced through the food chain to pigs (Molbak et al., 1999).
In the same year an outbreak of multiresistant S. Typhimurium DT 104 in the UK, involving
over 200 persons, and in which the vehicle of infection was milk, was traced to the farm of
origin (Walker et al., 2000). In all three examples, the causative organism was isolated from the
food animal, from foods, and from patients.
To some extent antimicrobial resistance in Salmonella is serotype-dependent, with resistance
and multiple resistance common in serotypes such as Typhimurium, Virchow, Derby and
Newport (Threlfall et al., 2000a; Varma et al., 2006) and more recently Hadar (Threlfall et al.,
2003) and Paratyphi B variant Java (Miko et al., 2003; Evans et al., 2005; Threlfall et al.,
2005). In contrast, other serotypes important for public health, for example S. Enteriditis rarely
display multiple resistance although resistance to antimicrobials such as nalidixic acid and
ciprofloxacin is increasing in incidence, with over 20 % of isolates in infections within EU
Member States from 2000-2005 exhibiting such resistance (Meakins et al., 2008).
Salmonella Typhimurium definitive phage type (DT) 104 is a multiresistant phage type with
almost global epidemicity. Since first identified in the late 1980s in the UK (Threlfall, 2000)
the organism has caused outbreaks in many countries throughout the world, with a variety of
food associations (Molbak et al., 1999; Walker et al., 2000; Threlfall, 2000; Horby et al., 2003).
Although declining in incidence in Europe, this S. Typhimurium strain remains a significant
public health hazard world-wide.
The strain is typically penta-resistant (ampicillin, chloramphenicol/florfenicol,
streptomycin/spectinomycin, sulphonamides and tetracyclines (ACSSuT)), resistance encoded
within a mobile genetic element designated Salmonella Genomic Island-1 (SGI-1). SGI-1 has
also been identified in other Typhimurium phage types, as well as at least 10 other Salmonella
serotypes including Agona, Albany, Newport and Paratyphi B variant Java.
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A further multiresistant strain which has been associated with international food-borne
outbreaks is S. Typhimurium DT 204b with resistance to up to 9 antimicrobial drugs. In 2000
the strain was responsible for at least one major international outbreak involving 10 countries
epidemiologically-linked to contaminated salad vegetables (Crook et al., 2003).
Extended spectrum beta-lactamase (ESBL) resistance has recently arisen worldwide in
Salmonella. Strains exhibiting such resistance have been detected in both humans and animals
(Bertrand et al., 2006; EMEA, 2008). In Belgium, a cephalosporin-resistant Salmonella
Virchow clone was found throughout the food chain. A similar spread was demonstrated for
cephalosporin-resistant S. Infantis. In this case, ESBL resistance was located on a conjugative
plasmid that had already spread to some other serotypes, including Paratyphi B variant Java and
Typhimurium (Bertrand et al., 2006; Cloeckaert et al., 2007).
4.1.1.2. Exposure through foods
The occurrence of antimicrobial-resistant Salmonella spp. in pig meat in five Member States
(MS) has been reported (EFSA, 2006b). The proportion of isolates reported (serotypes mostly
unspecified, but including Derby, Enteritidis, Infantis, London, Saintpaul, Senftenberg,
Typhimurium and Virchow) to be resistant to ampicillin in each of the five MS ranged from
21% to 35%, while resistance to sulphonamides (36 % to 52%) and tetracycline (38% to 59%)
was also common. Resistance to ciprofloxacin was reported in 1% of isolates in Denmark, and
resistance to enrofloxacin was reported in 0.6% of isolates by Italy. No data was reported for
the other MS. In the UK, studies of shell eggs coordinated by the Food Standards Agency have
demonstrated a substantive level of resistance in S. Enteritidis (most were resistant to nalidixic
acid with reduced susceptibility to ciprofloxacin) isolated from eggs imported into the UK, but
little if any resistance in isolates of S. Enteritidis from home-produced eggs (FSA, 2006).
Similarly, studies of organisms from raw red meats in the UK has demonstrated contamination
of beef, lamb and pork with a range of multiresistant S. Typhimurium phage types, with DT 104
and related strains predominating, whilst resistance was rare in other serotypes (Little et al.,
2008).
4.1.1.3. Reports linking foodborne AMR Salmonella to human infections
The EFSA report on source attribution for human salmonellosis in meat summarises the
findings from 5 attribution studies (EFSA, 2008b). This summary indicates that the proportion
of foodborne cases varies, but is around 90 - 95% of cases. In the EU, amongst the foodborne
cases, eggs, and egg products are the most frequently implicated sources. Meat is also an
important source, with poultry and pork implicated more often than beef and lamb. The main
food sources of Salmonella outbreaks in the UK are desserts (26%); poultry (25%); red meat
(14%) and eggs (13%) (Adak, 2005). Results from a Dutch case-control study for S. Enteritidis
and S. Typhimuium do not contradict the outbreak sources given above (Doorduyn et al., 2006).
Doorduyn et al. (2006) found that for S. Enteritidis, consumption of raw eggs and products
containing raw eggs were identified as risk factors (which may correspond to the 26% of
outbreaks caused by the consumption of desserts in the UK study). Similarly for S.
Typhimurium, occupational exposure to raw meat and the consumption of raw meat were
identified as risk factors.
In a US FoodNet case-control study of sporadic multiple-resistant Salmonella Newport
infections Varma et al. (2006) concluded that patients were more likely to have consumed
uncooked ground beef or runny scrambled eggs or omelettes prepared in the home. Travel was
not a risk factor for multiple-resistant S. Newport. Earlier studies (including outbreak
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investigations) for the same hazard, incriminated consumption of ground beef, ground horse
meat and cheeses made from nonpasteurised milk. In the published literature, contaminated
milk (Olsen et al., 2004), lettuce (Horby et al., 2003), dried anchovy (Ling et al., 2002) and
raw-milk cheese (Cody et al., 1999, Villar et al., 1999) among other foods have all been
identified as food vehicles for outbreaks of multidrug-resistant Salmonella Typhimurium.
Microbial sub-typing can provide useful information during outbreak investigations but also at
a population level. Isolates derived from humans, animals and food are obtained, analysed
using a discriminatory method and are finally compared. This procedure has become popular as
an attribution method for non-typhoidal Salmonella due to the fact that particular Salmonella
serotypes are more likely to be observed in certain animals and/or foods. Using such
information and routine surveillance data, attribution is routinely undertaken in both the
Netherlands (Van Pelt et al., 1999) and Denmark (Hald et al., 2004) using statistical models.
Using this approach, the main sources of Salmonella are identified to be eggs and pork in The
Netherlands and table-eggs, pork and imported chicken in Denmark. In an extension of the
study by Hald et al. attribution of antimicrobial-resistant Salmonella related cases has also been
investigated (Hald et al., 2007). In this study they considered the attribution of resistant, multiresistant and quinolone-resistant strains and concluded that (a) imported poultry and Danish
eggs were important sources for quinolone-resistant Salmonella, (b) pork (Danish and
imported) and imported beef for multidrug-resistant Salmonella infections and (c) Danish pork
for resistant Salmonella infections. Also, (d) travel was associated with the acquisition by
consumers, of multi-resistant and quinolone-resistant Salmonella strains.
4.1.2.
Typhoidal Salmonella
4.1.2.1. Hazard identification and characterisation
Typhoid fever, sometimes known as enteric fever, is a disease caused by the bacterium
Salmonella enterica serotype Typhi. Typhoid fever is a serious disease which can be lifethreatening unless treated promptly with appropriate antimicrobials, which may be necessary
before the results of laboratory sensitivity tests are available. The disease varies in severity, but
nearly all patients experience fever and headache. Slightly less serious, but nevertheless very
debilitating and possibly fatal, is enteric fever resulting from infections with Salmonella
Paratyphi A. Again, appropriate antimicrobial treatment is essential and should be commenced
as soon as the disease is diagnosed. The first-line antimicrobials of choice for infections with
both Salmonella Typhi and Paratyphi A are fluoroquinolones such as ciprofloxacin, with thirdgeneration cephalosporins and azithromycin as possible alternatives, particularly when the
causative strains are resistant to the first-line antimicrobial. Both Salmonella Typhi and
Paratyphi A are not indigenous to Member States, and the majority of infections are linked to
travel to endemic areas such as the Indian sub-continent, Africa, or south and central America.
Antimicrobial resistance to therapeutically important antimicrobials is of major concern, and
strains with resistance or decreased susceptibility to antimicrobials such as ciprofloxacin are
becoming widespread in developing countries, particularly the Indian sub-continent and
consequently in travellers returning from these areas to Member States and elsewhere (Threlfall
et al., 2008).
4.1.2.2. Exposure through foods
Salmonella Typhi and Paratyphi A do not have a food animal reservoir and infections are for
the most part spread by eating food or drinking beverages that have been improperly handled by
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an infected person, or by drinking water that has been contaminated by sewage containing the
bacteria.
4.1.2.3. Reports linking foodborne AMR Salmonella Typhi to human infections
Substantive outbreaks of typhoid fever in developing countries caused by drug-resistant strains
have been reported as a result of contamination of water supplies, with significant mortality
(Mermin et al., 1999), which clearly demonstrates the importance of sanitation and an
unpolluted water supply.
4.1.3.
Thermophilic Campylobacter
4.1.3.1. Hazard identification and characterization
In recent years in the European Union, Campylobacter has been the most commonly reported
diarrhoeal bacterial zoonotic pathogen (EFSA 2005b, 2006b). Most infections are caused by
Campylobacter jejuni and Campylobacter coli of which C. jejuni accounts for the vast majority
(>95%) of infections. Patients usually recover without antimicrobial therapy, but in some
patients with severe, prolonged, or relapsing illness such therapy may be indicated. Macrolides
are normally considered the drug of choice, but fluoroquinolones are also recommended (Blaser
1990; Goodman et al., 1990; Petruccelli, et al., 1992; Salazar-Lindo, et al., 1986; Skirrow and
Blaser, 2002). In a recent study of eleven randomised controlled trials of antibiotic treatment
versus placebo in patients with Campylobacter infections, antibiotic treatment with
erythromycin or fluoroquinolones significantly shortened the duration of intestinal symptoms
(Ternhag et al., 2007). Increases in the occurrence of Campylobacter causing infections in man
that are resistant to macrolides and fluoroquinolones have been reported in several countries
(Endtz et al., 1991; Rautelin, et al., 1991; Reina et al., 1994; Sanchez et al., 1994; Gaudreau
and Gilbert, 1998; Sjøgren et al., 1997; Hoge et al., 1998; Smith et al., 1999). As food animals
are considered one of the most important sources of Campylobacter causing infections in man,
the development of antimicrobial resistance in Campylobacter spp., due to the use of antimicrobial agents in food animals, is therefore a matter of concern should antimicrobial therapy be
indicated.
Several studies have shown that infections with fluoroquinolone-resistant Campylobacter in
humans are associated with adverse effects for human health, mainly measured by prolonged
diarrhoea (Smith et al., 1999; Helms et al., 2005; Engberg et al., 2004; Nelson et al., 2004;
Campylobacter sentinel, 2002). Although the results of these studies are not all statistically
significant they point in the same direction and taken together they suggest that there is a longer
duration of illness in patients infected with fluoroquinolone-resistant strains. In addition, it has
been shown that there is an increased risk of death or invasive illness following an infection
with a fluoroquinolone- or macrolide-resistant Campylobacter compared to susceptible strains
(Helms et al., 2005). The effect of macrolide resistance on human health consequences have
only been estimated in this one study and the results require to be verified in additional studies.
In contrast a critical examination of available data by Wassenaar et al. (2007) has suggested that
fluoroquinolone-resistant Campylobacter infections are not more severe than those caused by
susceptible strains.
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4.1.3.2. Exposure through foods
Thermophilic Campylobacter, especially C. jejuni and C. coli are normal inhabitants of the
gastrointestinal tract of most warm-blooded animals including the major food-animals cattle,
swine and poultry. Surveys of the faeces of healthy cattle and swine consistently show high
isolation rates, often above 50%, but the actual carrier rate in food-animals is likely to be higher
due to limitations in detection methods. Surveys of poultry, notably chicken, turkeys, ducks and
geese, indicate large variations in the proportions of flocks that are infected. The large variation
depends on the type of production system, the geographical location and on the time of year
(season).
Because Campylobacter is often present in animal faeces, Campylobacter can be found where
faeces contamination occurs. During evisceration, particularly of poultry, when the intestines
and other internal organs are being removed, some degree of faecal contamination is inevitable
no matter how stringent the hygiene measures that are applied. It is however important to note
that, following evisceration, the Campylobacter present on carcasses do not multiply further.
They may, however, be passed on to other products by cross-contamination. The rate by which
Campylobacter dies in the food processing and food distribution system depends on many
factors. The most important factors are temperature, oxygen tension and water activity (aw)
(Tomancova et al., 1991; Lee et al., 1998; Bhaduriand Cottrell, 2004). The potential
transmission of Campylobacter along the food chain greatly depends on the contribution of
each of the different processing steps from slaughter to meat packing.
Freezing or chilling of poultry meats has been shown to greatly reduce the number of live
Campylobacter including AMR Campylobacter present on the product.
There are no significant biological reasons why resistant Campylobacter should not transmit
equally well from animals to humans, as does sensitive Campylobacter. A temporal association
between resistance emergence and its increase in animals and humans following the
introduction of the antimicrobial in animal production has been shown by several studies
(Endtz et al., 1991; Smith et al., 1999; Engberg et al., 2001). In addition, results of a further
study have indicated that that certain strains gain increased fitness, as defined by Luo et al.
(2005), when acquiring fluoroquinolone resistance mutations (Luo et al., 2005).
Most studies conducted in several countries have identified poultry (especially consumption of
undercooked chicken) as the main risk factor for sporadic campylobacteriosis (Wingstrand et
al., 2006). Additional risk factors include foreign travel, drinking contaminated water or milk,
barbecuing, swimming in contaminated water and contact with pet animals. Other
epidemiological data also identify poultry as the main reservoir of human campylobacteriosis.
Development of AMR in C. jejuni and C. coli has important public health implications. Food
is a recognized vehicle through which exposure can occur. Several studies have examined the
occurrence of Campylobacter in various food categories (Meldrum and Wilson, 2007; Mena et
al., 2008; Roasto et al., 2007). In a study reported from Korea, 770 retail raw meat samples
were investigated for multi-drug resistant Campylobacter and these data demonstrated the
widespread nature of the organism (Hong et al., 2007). Levesque et al., (2007) compared
Campylobacter jejuni isolates from humans, with those recovered from various foods,
including chicken, raw milk and the environment. Isolates from chickens were resistant to
erythromycin, a feature that could lead to treatment failure in humans.
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Foodborne Antimicrobial Resistance
4.1.3.3. Reports linking foodborne AMR Campylobacter to human infections
A number of case-control studies have specifically addressed risk factors for fluoroquinoloneresistant Campylobacter. Examples include those by Smith et al. (1999); The Campylobacter
Sentinel Surveillance Scheme Collaborators (2002); Engberg et al. (2004); Kassenborg et al.
(2004); Nelson et al. (2004) and Johnson et al. (2008). All of these case-control studies
identified foreign travel as a risk factor for acquisition of a fluoroquinolone-resistant
Campylobacter infection. In most of the studies, it is not possible to conclusively say what the
exposure food-stuff/route might have been when travellers visited these countries, although the
Campylobacter sentinel study identified consumption of chicken and bottled water as risk
factors for travel-related cases. Risk factors for non-travel related cases of fluoroquinoloneresistant Campylobacter were as follows: use of a fluoroquinolone before the collection of the
stool specimen (Smith et al., 1999); consumption of cold meat (precooked) (The
Campylobacter Sentinel Surveillance Scheme Collaborators 2002); consumption of fresh
poultry other than chicken and turkey (Engberg et al., 2004); swimming (pool, ocean, lake or
other places) (Engberg et al., 2004); consumption of chicken or turkey cooked at a commercial
establishment (Kassenborg et al., 2004) and possession of non-prescribed antimicrobials
(Johnson et al., 2008).
In Norway, the prevalence of fluoroquinolone resistance among C. jejuni isolates from
imported and indigenous sporadic human cases of campylobacteriosis and from domestic
broilers was assessed (Norström et al., 2005). Among the imported human isolates, 67.4% were
resistant to ciprofloxacin compared with 6.5% of indigenous human isolates. The prevalence of
resistance in indigenous human isolates was comparable with the prevalence of resistance in
isolates from Norwegian broilers (1.2% fluoroquinolone resistant). No quinolone preparations
are licensed for use in broilers in Norway
4.1.4.
Verotoxigenic Escherichia coli (VTEC) of public health concern
4.1.4.1. Hazard identification and characterization
Verotoxigenic Escherichia coli (VTEC) has emerged as a public health threat since its
identification in 1982 following an outbreak in the USA associated with the consumption of
contaminated ground (minced) beef (Riley et al., 1983). Escherichia coli O157:H7 and
O157:NM (non-motile) are major aetiological agents in hemorrhagic colitis (HC) and hemolytic
uremic syndrome (HUS) in humans (Mead and Griffin, 1998). Currently more than 200 E. coli
serotypes are recognized, and these have been isolated from animals, food and other sources.
Of these, only 60 serotypes have been linked with human disease. In the US, the Centres for
Disease Control & Prevention (CDC) estimate that E. coli O157:H7 causes approximately
73,400 illnesses and 60 deaths each year (Mahon et al., 1997; Mead et al., 1999).
Bovines are a major VTEC reservoir and resistant strains may colonise the human population
via the food chain. Earlier reports signalled an increase in antimicrobial resistance among
O157 and non-O157 serotypes (Aarestrup and Wagner, 1999; Farina et al., 1996; Kim et al.,
1994; Threlfall et al., 2000b; Schroeder et al., 2002; White, 2002) whilst others suggested that
the occurrence of antimicrobial resistance among three VTEC serotypes was low (Walsh et al.,
2006).
The use of antimicrobials for the treatment of human infections with VTEC is controversial. In
general, antimicrobials are not recommended as their usage may exacerbate symptoms,
particularly haemolytic uraemic syndrome. Antimicrobials may be of use in the early stage of
The EFSA Journal (2008) 765, 22-87
Foodborne Antimicrobial Resistance
infection and in some countries, fosfomycin has been used for treatment, with some success
(Igarashi, 2002).
4.1.4.2. Exposure through foods
Food products derived from bovines can represent a source from which these pathogens can
enter the food chain. Schroeder et al. (2002) described the characterization of 27 E. coli
cultured directly from food (including beef, pork and unspecified sources), of which 17 were
defined as VTEC based on the presence of stx1 and/or stx2 markers. Among these isolates 26%
were resistant to sulfamethoxazole and a similar percentage was resistant to tetracycline. Apart
from these two drug classes, the majority of isolates were susceptible to the complete panel of
antimicrobials tested. Interestingly when VTEC and non-VTEC isolates were compared,
resistance among the latter was higher, although both were susceptible to third generation
cephalosporins (ceftriaxone and ceftiofur).Whereas in a study by Klein and Bülte (2003) in
Germany no multiresistant VTEC isolates could be identified, another study recently showed
more than 50% of porcine VTEC isolates and 25% of bovine isolates as multiresistant in
Germany (von Müffling et al., 2007). In both studies resistance to tetracyclines was most
common.
Herd-level surveillance among dairy animal populations is a convenient way to assess the risk
of pathogen transmission through milk (Murphy et al., 2005). Using this approach, over a twoyear period, 16 VTEC strains were recovered from animals supplying raw milk for the
manufacture of cheese. With the exception of one isolate, resistant to streptomycin, all were
susceptible to the panel of drugs tested. In a more recent study (Murphy et al., 2007), baseline
data were obtained on the prevalence and characteristics of VTEC microorganisms in lactating
animals (bovines, ovines and caprines) supplying milk to the farmhouse cheese sector and for
the manufacture of raw milk ice cream. Milk samples were analysed for the presence of
serotypes O111, O157 and O26 and the susceptibility patterns determined. No O111 serotype
was recovered. All of the O157 isolates were susceptible to the panel of 15 antimicrobials
tested and among the O26 isolates, three (of 17) were defined as multi-drug resistant, a further
three resistant to ampicillin, three more were resistant to tetracycline and only one isolate was
resistant to streptomycin. The genetic basis of resistance was not examined in these studies.
There is a paucity of information regarding the mechanisms of antimicrobial resistance among
VTEC strains. In a study of 274 VTEC strains (recovered from poultry, bovines, swine and
humans) class 1 integrons were detected in 16% of the study population (Singh et al., 2005).
These structures facilitate the emergence and dissemination of antimicrobial resistance among
strains independent of origin. Similarly, in a study of 105 epidemiologically-unrelated VTEC
strains belonging to serogroup O111 from humans and cattle isolated in Germany between 1983
and 2003, resistance was detected in 76 % of isolates mediated by a range of resistance genes
including those coding for resistance to ampicillin, chloramphenicol, aminoglycosides,
tetrcyclines and trimethoprim (Guerra et al., 2006). It is acknowledged that the emergence of
resistance among these strains may further limit therapeutic options.
4.1.4.3. Reports linking foodborne AMR VTEC to human infections
Comparisons between non-VTEC and VTEC isolates from food animals and both symptomatic
and asymptomatic humans, showed that the former appear to display a broader resistance
profile (Bettelheim et al., 2003). Nevertheless, whilst resistance among VTEC strains is still
relatively low, (Walsh et al., 2006) surveillance will be important to recognize any future
changes in these early trends. One report described antimicrobial resistance in VTEC strains (4
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Foodborne Antimicrobial Resistance
of 59 isolates examined or 6.8%), cultured from patients presenting with diarrhoea and urinary
tract infection (UTI) to common antimicrobials including ampicillin and tetracycline (Banerjee
et al., 1999). Murphy et al., (2007) similarly reported the identification of multiple-resistant
strains recovered from bovine milk used in the production of farmhouse cheese (Murphy,
2007); however, it is not known if any of these isolates caused human infection. In VTEC
strains isolated in Bosnia and Germany, all were resistant to sulphonamide, many of the porcine
isolates were resistant to oxy- and chlortetracycline, and bovine isolates were resistant to
sulphonamide/trimethoprim and ampicillin (von Muffling et al., 2007).
4.1.5.
Shigella
4.1.5.1. Hazard identification and characterization
The normal presentation of bacillary dysentery caused by strains of Shigella of subgroups A, B,
C (Shigella dysenteriae, Sh. flexneri, Sh. boydii) and D (Sh. sonnei) is that of mild to moderate
gastroenteritis. The disease is self-limiting and the primary therapy is oral rehydration.
However, symptoms can be severe in the very young, the very old, the malnourished, and
patients with other underlying diseases. In such cases, administration of an effective
antimicrobial should commence as soon as clinical diagnosis is made. Ampicillin was the
antimicrobial of choice until the mid-1980s. Following the widespread emergence of
ampicillin-resistant strains this antimicrobial was compromised and was replaced by cotrimoxazole (trimethoprim plus sulphamethoxazole) and nalidixic acid as the first-line drugs.
More recently, the American Public Health Association have recommended that, should
antimicrobial therapy be indicated for cases of acute shigellosis, then oral trimethoprimsulphamethoxazole, ciprofloxacin or ofloxacin should be used for adults and oral trimethoprimsulphamethoxazole, nalidixic acid or parenteral ceftriaxone for children (Chin, 2000).
Within the European Union infections with Shigella dysenteriae, Sh. flexneri, Sh. boydii are
normally associated with travel to countries outside Europe, particularly the Indian subcontinent, Africa and south and central America. Infections with Sh. sonnei are indigenous in
many European countries (Cheasty et al., 2004).
4.1.5.2. Exposure through foods
Although being a foodborne pathogen, shigellae are not considered to have a food animal
reservoir and infections are normally a result of person-to person transmission. However,
contamination of foods or water by human faecal material has led to human cases. Foods
implicated in human cases of shigellosis include fresh fruit and vegetables, raw oysters, deli
meats and unpasteurized milk
4.1.5.3. Reports linking foodborne AMR Shigella to human infections
Certain food products which have been subjected to contamination by human sewage and that
have been responsible for national or international outbreaks have been linked to AMR
Shigella. Seafood has been particularly implicated and of note have been oysters (Terajima et
al., 2004) and ready-to-eat shrimps (Duran and Marshall, 2005). In 2007 imported baby corn
originating from Thailand was linked to drug-resistant shigellosis cases in Australia, and to an
outbreak involving more than 100 persons in Denmark (Stafford et al., 2007). In all the above
outbreaks the causative organism was Sh. sonnei.
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Foodborne Antimicrobial Resistance
4.1.6.
Vibrio
4.1.6.1. Hazard identification and characterization
As with Shigella, infections with Vibrio spp. are normally the result of contamination of food
and water with human faecal material. The standard treatment in such cases is oral rehydration,
but should antimicrobials be required, then tetracyclines have for many years been the first-line
choice. More recently, because of the emergence of strains with resistance to tetracyclines,
fluoroquinolones have been used when treatment has been indicated.
Recently the efficacy of fluoroquinolones has been jeopardised following the emergence of
resistant strains in the Indian sub-continent and Europe. There is no evidence to suggest that the
emergence of resistance to critical antimicrobials in V. cholerae is linked to the use of
antimicrobials in food production animals.
4.1.6.2. Exposure through foods
Vibrio cholerae serogroups O1, O139 and non-O1/non-O139 are not considered to have a
traditional food animal reservoir. Infections result from the ingestion of faecally contaminated
water or food in the case of cholera, or the consumption of seafood such as shrimp (Duran and
Marshall 2005; Boinapally and Jiang 2007), and cockles or oysters in the case of V.
parahaemolyticus. This is due to the the fact that the principal reservoir for these bacteria is the
aquatic environment. When such strains have been antimicrobial-resistant, then infections or
substantive outbreaks with resistant strains have resulted (Weber et al., 1994). Though V.
vulnificus has been obtained from a number of sources in inshore marine areas, the significant
food contamination is of shellfish and particularly of oysters. The vibrio is very heat sensitive
and has not been reported on processed foods (ICMSF, 2005; Bang and Drake, 2002; Kim et
al., 1997)
4.1.6.3. Reports linking foodborne AMR Vibrio spp. to human infections
A variety of food products have been involved in foodborne AMR Vibrio outbreaks, most often
seafood and seafood products. The causative agent was V. parahaemolyticus, and up to 10% of
the isolates were multi-resistant (Wong et al., 2000). A case control study identified V. cholerae
as a source of foodborne infection, with 36% of the isolates being multi-resistant. In particular,
raw seafood, unboiled water or cooked crabs were identified as associated with illness (Weber
et al., 1994). Virtually all reported V. vulnificus food borne cases have resulted from
consumption of raw oysters by susceptible individuals with no information about AMR
(ICMSF, 2005).
4.1.7.
Meticillin11-resistant Staphylococcus aureus (MRSA)
Staphylococcus aureus is a bacterium found on the skin or in the nostrils of humans. The
bacterium is carried temporarily and rarely poses a problem for people in full health, although it
is a major cause of nosocomial infections, often causing postsurgical wound infections. Some
strains are capable of producing an enterotoxin that can cause foodborne intoxication.
Meticillin-resistant Staphylococcus aureus (MRSA) has a generally decreased sensitivity to βlactam antimicrobials, and is thus a serious clinical problem in hospital environments. The
resistance is based on a specific penicillin-binding protein, PBP2’ (or PBP2a), coded by mecA
11
Meticilin (International Nonproprietry Name) = Methicillin (United States Adopted Name)
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Foodborne Antimicrobial Resistance
(Hartman and Tomasz, 1984). The mecA gene is typically part of an integron associated with
the S. aureus chromosome (Katayama et al, 2000).
From being considered as almost exclusively a nosocomial pathogen, MRSA has during the last
two decades emerged in the community. Furthermore, it has recently also caused infections in,
and colonized, domestic pets and food production animals. MRSA has been detected in cattle,
chickens, horses, pigs, dogs, rabbits, seals, birds and cats. The colonization in animals has in
several cases been implicated in infections in humans and infection with MRSA may today be
considered as a zoonosis. It is, important to distinguish between the epidemiology of MRSA in
relation to production animals, where a new clone appears to be emerging, and pet animals
infected with classical human variants of MRSA (Manian, 2003; Weese et al., 2006).
4.1.7.1. Hazard identification and characterisation
Meticillin-resistant Staphylococcus aureus (MRSA) has been identified amongst pig farmers,
and abattoir workers, indicating, in this instance, not a food hazard but an occupational hazard.
Multilocus sequence typing indicates that there is a common type. However, MRSA which has
also been identified on meat, (Kitai et al., 2005; van Loo et al., 2007b; Normanno et al., 2007,
VWA, 2008), may be a hazard as a consequence of handling contaminated meat. JuhaszKaszanyitzky et al. (2007) reported subclinical MRSA mastitis in dairy cattle. Milk derived
from cows with subclinical MRSA mastitis may be considered as a source of MRSA in milk.
One specific clone (ST398) has been found in several countries including Austria, Belgium,
Canada, Denmark, France, Germany, The Netherlands and Singapore where it has been isolated
from both production animals and humans (van Loo et al., 2007a, b; Tan et al., 1994; Wijaya et
al., 2006). Surveys in Sweden and Switzerland were negative. With our current knowledge it
seems quite evident that ST398 is a MRSA clone transmitted from production animals to
humans. Its origin is currently unknown. Further studies are underway in several countries, but
it seems likely that MRSA ST398 is widespread in the food animal population, most likely in
all Member States with intensive animal production. For example, a study in Germany found a
prevalence of MRSA of 12.5% of 678 isolates from pigs in 17.9% of the 62 farms investigated,
all of the isolates being typed as ST398 (Blaha, 2008). A recent study from the Netherlands
found MRSA in small quantities in turkey (31%) of samples), chicken (27%), veal (17%), pork
(10%), beef (10%) and lamb (6%) meats at retail. Most (84%) of the MRSA found was to be
ST398 (VWA, 2008). The reason for the colonization of MRSA ST398 in pigs and other
production animals and the epidemiology of this clone are currently not known; it possibly first
emerged in 2003, as it was not detected in 2002 in the human monitoring done in Holland, or in
monitoring from 1992-2003 of human isolates in Germany.
Case-control studies in both Denmark and The Netherlands have shown that the people at risk
of being colonised with ST398 are those persons working or living on farms and mainly those
in direct contact with animals (van Loo et al., 2007). This is also underlined by the above
mentioned German study (Blaha, 2008) who found that people working with live animals on
farms showed a higher rate of nasal contamination (41.8%) than those working in
slaughterhouses or in diagnostic laboratories (13.4% of a total of 86 persons investigated). All
positive isolates were ST398.
A baseline study on the prevalence of MRSA in holdings of breeder pigs is now being carried
out across Member States12 (EFSA, 2007b), and an assessment by EFSA of the public health
significance of MRSA in animals and foods (EFSA-Q-2008-300) is being prepared.
12
OJ, L 14, 17.1.2008, p10-25
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Foodborne Antimicrobial Resistance
4.1.7.2. Exposure through foods
In Korean studies, MRSA has been frequently isolated from food producing animals, albeit at a
relatively low frequency. While the study of Lee (2003) indicated the few animal isolates were
closely related to human isolates, the studies of Kwon et al. (2005, 2006) suggested that isolates
from bovine milk had a different subtype of the resistance cassette and might not be related to
community-acquired human cases nor to the ST398 clone recently identified in Europe. Two
Japanese poultry-associated MRSAs shared the characteristics of community-acquired human
MRSA-strains (Kitai et al., 2004).
In an Italian study, MRSAs were found at a frequency of 3.75% in S. aureus isolates derived
from different foods of animal origin. Four isolates were from bovine milk and two from dairy
products (pecorino and mozzarella cheese). The strains were able to produce enterotoxins, but
no association with cases of food poisoning nor to relatedness to human MRSA isolates was
made (Normanno et al., 2007).
4.1.7.3. Reports linking foodborne MRSA to human infections
The first food-associated MRSA outbreak resulting in several fatalities was described by
Kluytmans et al. in 1995. The origin was most likely a colonized health care worker (HCW)
who was responsible for preparing the food for haematology patients. Identical strains were
isolated from the HCW, a food item (peeled banana) and from the first patient involved in the
outbreak. The HCW had no direct contact with patients. Airborne transmission was thought to
play an important role in the subsequent spread of the outbreak. Jones et al. (2002), reported a
small outbreak involving a family which had consumed a contaminated meal purchased from a
delicatessen. The origin of this outbreak was most likely also human. Further outbreaks have
apparently not been reported. However, animal products remain a potential source of MRSA.
Food-associated MRSA, therefore, may now be an emerging problem.
4.1.8.
Listeria monocytogenes
4.1.8.1. Hazard identification and characterisation
Foods associated with transmission of Listeria monocytogenes to humans become contaminated
either at source (e.g. from the general environment), from sites within food production
environments, or by cross-contamination during subsequent stages in the food chain. Penicillin,
ampicillin, amoxicillin with or without gentamicin or trimethoprim-sulfamethoxazole (TMPSMX) are recommended for the treatment of listeriosis. Although plasmids conferring
resistance to tetracyclines, chloramphenicol, macrolides, streptomycin and trimethoprim have
been described, all strains are susceptible to these antimicrobial agents or combinations of such.
All strains of L. monocytogenes are intrinsically highly resistant to cephalosporins (Johnson et
al., 1996; Threlfall et al., 1998; Hansen et al., 2005); this may present therapeutic problems if
this class of antimicrobial agent is used for blind therapy (therapy in the absence of
confirmation of the causative agent of infection).
There is relatively little evidence for emergence of antimicrobial resistance in the bacterium;
indeed the resistance pattern has remained virtually unchanged for the past 40 years (Johnson et
al., 1996; Threlfall et al., 1998; Charpentier and Courvalin, 1999; Hansen et al., 2005).
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Foodborne Antimicrobial Resistance
4.1.8.2. Exposure through foods
Transmission of L. monocytogenes occurs through several routes; however the majority of cases
are considered to occur as a result of eating contaminated food (McLauchlin 1996).
4.1.8.3. Reports linking foodborne AMR L. monocytogenes to human infection.
Epidemiological analysis of both sporadic cases and outbreaks of human listeriosis have shown
that the foods associated with transmission are predominantly ready-to-eat foods, with those
extended (usually refrigerated) shelf-life foods capable of supporting the growth of L.
monocytogenes (McLauchlin, 1996) being of particular importance. Antimicrobial resistance is
not a therapeutic problem for the treatment of listeriosis; this situation may be reversed if
resistance develops or horizontal transfer of key resistance genes occurs. It should be
emphasied that there are no reports linking foodborne L. monocytogenes with antimicrobial
drug resistance to cases of human infection.
4.2.
Commensals
Commensal bacteria are those bacteria that live in or upon the host without causing disease.
Mostly, this co-existence is of mutual benefit. However, many commensals can cause disease if
they enter body sites that are normally sterile or when the host’s immune defence is impaired
(Sharp, 1999). As discussed in Section 3.7, commensal bacteria that contaminate food can
harbour transferable resistance genes. During the passage through the intestine, these bacteria
may transfer their resistance genes to host-adapted bacteria or to pathogens. Exchange of
resistance genes between bacteria from different sources can also occur in the kitchen
environment (Kruse and Sørum, 1994; Walsh et al., 2008). The most studied species are
commensal Escherichia coli and Enterococcus spp.
4.2.1.
Escherichia coli
Commensal E. coli from the intestines of animals and humans contaminate foods of animal
origin, vegetables and water and may carry transferable resistance genes (Sunde and Norström,
2006). One of the best documented specific examples of spread of resistance genes from
animal to human bacteria is transposon-encoded streptothricin resistance (Tschäpe, 1994).
Following the introduction of norseothricin for use as a growth promoter in pig production,
resistance emerged in commensal E. coli of pigs and farmers, and later in urinary isolates of
Salmonella, and in E. coli and Shigella causing disease in humans (Hummel et al., 1986;
Tschäpe, 1994). Another example is the spread of apramycin resistance, an antimicrobial used
exclusively in animals. Apramycin resistance was first described in E. coli and S. Typhimurium
from animals (Chaslus-Dancla et al., 1986; Wray et al., 1986) and has since been demonstrated
in various enterobacteria from animal, human and environmental sources (Chaslus-Dancla et
al., 1989; Hunter et al., 1994; Hunter et al., 1993; Threlfall et al., 1986).
4.2.1.1. Hazard identification and characterisation
Infections with multi-resistant Gram-negative bacteria are currently among the major challenges
in health-care settings in Europe and elsewhere. Gram-negative pathogens can be recipients of
resistance genes transferred from commensals such as E. coli and may cause serious infections
in, e.g. the blood-stream, abdomen, lungs and urinary tract and can lead to septicaemia
(Livermore et al., 2007). Meanwhile, multi-resistant E. coli are also increasingly associated
with urinary tract infections in the community (Calbo et al., 2006; Woodford et al., 2007).
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Foodborne Antimicrobial Resistance
4.2.1.2. Exposure through foods
Phenotypic data on resistance to antimicrobials in E. coli isolated from food have been
compiled from the summary report on zoonoses in the EU (EFSA, 2006b) and from national
reports on monitoring of resistance. Comparability is hampered by differences in inclusion
criteria, testing methodology and choice of interpretation criteria as the epidemiological cut-off
values were not uniformly used for compilation of some of the reports quoted (see 2.2.2).
Notwithstanding this, resistance to ampicillin, streptomycin, tetracyclines and trimethoprim is
common in E. coli from beef, poultry meat and pork. These antimicrobials are also those
frequently employed in animal husbandry for therapy and prophylaxis. A high proportion of
isolates resistant to fluoroquinolones is reported from poultry in some countries. Resistance to
3rd generation cephalosporins is still not common according to these reports, but The
Netherlands has reported a rapid increase in resistant isolates from broilers and broiler products
and Canada has reported very high figures, also from broilers (see Appendix, Table B).
4.2.1.3. Reports linking foodborne AMR E. coli to human infections
Most food-derived E. coli will be transient and non-pathogenic to the host. Resistance genes
may be transferred to host-adapted species or to zoonotic pathogens such as Salmonella, during
passage through the intestine or in food. Indeed, non-pathogenic multidrug-resistant E. coli in
the intestine are an important reservoir of resistance genes (Osterblad et al., 2000) and these E.
coli isolates of animal origin may colonize the human intestine at least temporarily (Linton et
al., 1977; Marshall et al., 1990; Orskov and Orskov, 1992). Transfer of resistance genes from E.
coli to Salmonella has been demonstrated experimentally in poultry intestinal tract (Gast and
Stephens, 1986, Poppe et al., 2005). Further, there are some reports indicating acquisition of
resistance plasmids by E. coli and Salmonella in the human gut (Su et al., 2003; Yan et al.,
2005). Exchange of resistance genes between bacterial clones has also been demonstrated
experimentally in water, soil, on kitchen towels, on cutting boards, and on the surface of food
(Kruse and Sørum, 1994; Walsh et al., 2008).
Spread of resistance genes between bacteria colonising animals and man has been shown. For
example, some studies have shown that the same R plasmids can be transferred between
bacterial strains from bovines and humans (Oppegaard et al., 2001). Some categories of food
may often be contaminated with E. coli, including resistant isolates (Sunde and Nordström,
2006), and these bacteria reside long enough in the intestines of humans to be able to transfer
resistance genes to the residential flora. It is therefore highly probable that food is a vehicle for
spread of resistance genes between different ecosystems.
4.2.2.
Enterococcus
Enterococci (former D streptococci or faecal streptococci) are natural commensals of the human
and animal gut. In addition, they occur in foods as contaminants but are also present as
acidifying microorganisms in many traditional and artisanal fermented products (Franz et al.,
2003) (See also 4.3).
Enterococci are intrinsically resistant to cephalosporins, low concentrations of
aminoglycosides, clindamycin, fluoroquinolones and trimethoprim-sulfamethoxazole. In
addition, many strains harbour transmissible genetic elements for acquired resistance for
various antimicrobials (tetracycline, erythromycin, chloramphenicol) (Cetinkaya et al., 2000).
The acquired resistance to glycopeptide antimicrobials (vancomycin, teicoplanin) has received
most attention, because of the rapid increase in the occurrence of vancomycin resistant Ent.
faecalis and Ent. faecium strains (VRE) both among clinical isolates and food and faecal strains
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Foodborne Antimicrobial Resistance
(Bates et al., 1994; Bates, 1997) since the first report of their isolation (Leclerq et al., 1988;
Uttley et al., 1989). While vancomycin resistance compromises the treatment of nosocomial
infections, there is an additional concern of the eventual transfer of the resistance to methicillinresistant staphylococci (MRSA), which would lead to extremely serious clinical consequences.
This transfer has been reported to occur under laboratory conditions (Noble et al., 1992), and
more recently clinical isolates of MRSA have also been found to harbour vancomycin resistant
genes, originating from enterococci (CDC, 2002).
4.2.2.1. Hazard identification and characterization
Since the 1970s, enterococci have become important agents in hospital-acquired infections,
causing mainly urinary tract and wound infections and endocarditis. The virulence factors
associated with enterococci include adhesins, invasions and hemolysin (Eaton and Gasson,
2001; Franz et al., 2003). The most common species detected in nosocomial infections is
Enterococcus faecalis. Occasionally also infections caused by Ent. faecium are encountered,
while clinical cases associated with other species (Ent. gallinarum, Ent. casseliflavus, Ent.
durans, Ent. avium, Ent. raffinosis) are rarely reported (Cetinkaya et al., 2000).
4.2.2.2. Exposure through foods
VREs can be isolated from animal faeces and from foods of animal origin (Wegener et al.,
1997; Bates, 1997; Klein, 2003; Eisner et al., 2005; Kaszanyitzky et al., 2007), and also from
healthy, non-hospitalized humans (Balzereit-Scheuerlein and Stephan, 2001). The former use of
a glycopeptide antimicrobial, avoparcin, as an antimicrobial growth promoter has contributed to
the formation of a reservoir of VRE in food-producing animals. Because of these concerns, the
growth promoter use of avoparcin has been restricted or banned in many third countries, and in
the EU since 1997.
Molecular studies indicate a high degree of clonality among the vancomycin resistance
determinants of animal origin. For example, an Ent. faecium-strain carrying a specific variant of
resistance transposon Tn1546 has been simultaneously detected in swine isolates from
Denmark, Spain, Portugal and Switzerland (Novais et al., 2005). In the studies of GarciaMigura et al. (2007a, b) the Tn1546 isolated from 19 unrelated farms show a very low diversity
of Tn types, while otherwise the genotypic diversity between the different farm isolates was
high. These findings suggest that horizontal transfer may have a more important role in the
persistence of vancomycin resistance than the clonal spread.
4.2.2.3. Reports linking foodborne AMR enterococci to human infections
There is little evidence of human infections being directly linked to the consumption of VREcontaminated foods. Apparently few, if any systematic studies on the prevalence of the known
enterococcal virulence factors among the food-associated VRE-strains have been done, while
generally the occurrence of virulence determinants in food isolates and in human commensals
appears to be low compared to clinical isolates (Eaton and Gasson, 2001; Franz et al., 2001;
Lempiäinen et al., 2005).
The question as to how frequently animal and food strains of enterococci can permanently
colonise humans, is to some extent an open one. Molecular studies indicate a certain overlap
between human isolates and strains from pigs and, to some extent, with isolates from poultry
and cattle (Bruinsma et al., 2002). In a Danish study the presence of a vancomycin-resistant
Ent. faecium, apparently related to the swine-associated clone mentioned above (Novais et al.,
The EFSA Journal (2008) 765, 30-87
Foodborne Antimicrobial Resistance
2005), has been detected in a healthy volunteer after seven years since the ban on avoparcin
usage (Hammerum et al., 2004).
The in vivo transfer of vanA genes from chicken isolates to human strains in human volunteers
has been detected (Lester et al., 2006), this being perhaps the strongest direct evidence of the
potential of animal strains to spread resistance to human strains with a resulting clinical
significance.
While the direct clinical infection in humans by VRE from food sources apparently is rare
although not totally excluded as a possibility, the reservoir of VRE in food-producing animals
presents a definite risk of resistance genes being transferred to virulent human strains through
food and other routes.
4.3.
Bacteria deliberately added to the food chain or being an integral part of the food
Fermentation is an ancient practice to improve the hygienic, nutritional and sensory quality of
perishable foodstuffs. Fermented foods all over the world are being prepared using
microorganisms that are either added as starter cultures, or, in more traditional or artisanal
production conditions, by back-slopping or relying on spontaneous fermentation in conditions
favouring the desired microbial community. The use of bacteria intended to promote the well
being of the host (probiotics) both in food and feed or the use of microbial preparation, as
protective cultures represent new ways by which deliberately added microorganisms enter the
food chain.
Microorganisms present in fermented food (see review of Wigley, 2000) are mainly lactic acid
bacteria (LAB). Typical food-associated LAB include members of the genera Lactobacillus,
Lactococcus, Leuconostoc and Pediococcus. Streptococcus thermophilus is a commonly used
species. In addition, enterococci occur in many traditional products, while some staphylococcal
and micrococcal species (S. carnosus, S. xylosus, M. varians) are used in certain meat
fermentations as colour and flavour producers. Propionic acid bacteria are typically added to
Emmenthal cheese. In probiotic food preparations LAB, often of intestinal origin (mainly
lactobacilli but also, particularly in feed applications, enterococci), or bifidobacteria, are
frequently used (Ouwehand et al., 2002).
4.3.1.
Hazard identification and characterisation
While occasional opportunistic infections caused by lactobacilli, usually associated with a
severe underlying disease, are reported (Gasser 1994; Salminen et al., 2006), no reports of
clinical cases associated with industrial starters have been found. A few cases of human
infections associated with a probiotic Lactobacillus rhamnosus strain have been described
(Rautio et al., 1999; de Groote el al., 2005). Considering the extensive use of this bacterium in
these products, these cases remain isolated incidents, and there have been no indications of
therapy failures due to any antimicrobial resistance in the strain.
There are relatively few studies on the prevalence of antimicrobial resistance markers in
currently used starter cultures, or in bacteria isolated from fermented foods. In an EU Sixth
Framework Program project ACE-ART, however, approximately 1400 isolates of lactic acid
bacteria and bifidobacteria of human, animal, food and feed origin were screened for typical
and atypical antibiotic resistances. Some of the results have already been published (Florez et
al., 2006, 2007; Korhonen et al., 2007; Mättö, et al., 2007; Tosi et al., 2007; Egervarn et al.,
2008). The general finding was that conspicuous transferable resistances were rare, and the
most common resistance occasionally detected was against tetracycline.
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Foodborne Antimicrobial Resistance
4.3.2.
Exposure through foods
While there has been no indication of widespread prevalence of antimicrobial resistance in
strains used as industrial starter cultures, there are studies indicating that antimicrobial-resistant
microorganisms can at least occasionally be isolated from fermented foods (Teuber et al., 1999)
or among probiotic strains (Masco et al., 2006).
In their review, Teuber et al. (1999) list a number of acquired antimicrobial resistances detected
in lactic acid bacteria isolated from foods. They most often occur among enterococci, which, in
addition to vancomycin resistance, can also harbour other resistance determinants, the most
common being genes associated with resistances to tetracycline, erythromycin and
chloramphenicol. These resistance determinants are often carried on conjugative plasmids,
which makes their transfer possible both among the enterococcal strains and even between
different bacterial genera.
As in the case of enterococci, lactococci and lactobacilli harbouring multiresistance plasmids
have been isolated from dairy products (Gfeller et al., 2003; Teuber et al., 1999). A high
incidence of tetracycline and erythromycin resistance determinants erm(B) and tet(S) were
detected among lactobacilli isolated from hand made artisanal cheeses in Turkey (Cataloluk and
Gogebakan, 2004). Tetracycline resistance determinants tet(M) and tet(S) have been found to
be relatively common in lactic acid bacteria associated with raw meat, while in the process of
preparation of fermented dry sausages tet(M) became dominant among the tetracycline resistant
isolates (Gevers et al., 2003).
In a recent study by Klare et al. (2007) 473 lactic acid bacteria strains representing nutritional or
probiotic strains or human and animal isolates were screened for antimicrobial resistance. Six
probiotic or nutritional cultures were found to be multi-resistant, possessing tet(W), tet(M) or
erm(B) determinants. In a study carried out in the USA (Wang et al., 2006) high incidences of
antimicrobial resistance were observed, particularly tet(S)/(M) and erm(B) markers in the
lactococcal and St. thermophilus isolates from retail dairy products, the frequency of resistant
strains ranging from 102 - 107 CFU g-1 food.
Antimicrobial resistance determinants including among others tet(W), have also been detected
in bifidobacteria, including seven Bifidobacterium animalis subsp. lactis and B. bifidum strains
used as probiotics (Masco et al., 2006).
4.3.3.
Antimicrobial-resistant starter and probiotic bacteria and human infections
While food-associated fermentative bacteria, whether antimicrobial-resistant or not (with the
possible exception of enterococci) do not present a clinical problem, they might act as a
reservoir of transmissible antimicrobial resistance determinants. Should strains with
transferable antimicrobial resistance genes become widespread in the food chain, the eventual
transfer of resistances to food associated or intestinal pathogens might become a possibility,
although the probability of such an event leading to actual clinical consequences is difficult to
evaluate. Nevertheless, avoiding the use of strains harbouring transmissible antimicrobial
resistance determinants in food or feed fermentation, or as probiotics is a prudent precaution
(von Wright, 2005), as reflected in the acceptance criteria of bacterial strains intended for use as
animal feed additives (SCAN, 2003; EFSA, 2005a).
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Foodborne Antimicrobial Resistance
5.
Categorisation of food with respect to risk of AMR
Major food categories to be considered include food of (1) animal origin including fish, (2)
plant origin, and (3) water used directly in the food chain. Mixed products are also considered,
as most ready-to-eat (RTE) foods and convenience products consist of foods of different origin
(e.g. pizzas, etc.). The latter category is included as one of the four main categories.
A further subdivision of food categories is concerned with the manufacturing process that has
been applied, i.e. if the products are offered at retail level and at the point of consumption as
fresh or raw, minimally processed or processed (i.e. heat treated or fermented) foods.
Several categorisation schemes for food exist (as for example, reviewed by Ireland and Moller,
2000), or are under development (e.g. EFSA13 and ISO14). These have been developed for
specific purposes. For the estimation of food consumption, data categories are usually defined
according to the nutritional value, taking into account the regional diversity of food. Other
listings concern the estimation of risk exposure to contaminants and residues; these follow lists
used for consumption data in order to estimate the amount of intake of specific food categories.
The categorisation used for the outbreak reporting in EFSA’s Zoonoses Report (EFSA 2006b,
2007d, e) refers to the origin of the food, i.e. animal species. These categories are useful for the
purpose of attribution of pathogens to products of animal origin. For the description of the role
of food in the dissemination of antimicrobial resistance these latter categories can be used in
part. The number of categories should not be too high; Additional information has also to be
considered, such as information about the manufacturing process used, as elucidated below. A
combination of these categorisation systems has been used here and is presented in Table 1.
Antimicrobial resistance is dependent on live microorgansims and the transfer of resistance
genes (see Chapter 3). Therefore any processing step that reduces or increases the bacterial load
has an influence on the risk of exposure to antimicrobial resistant bacteria. For the purpose of
this Opinion, food categories are defined according to their impact on bacterial survival and
growth. For different microorganisms different influences might apply, but in general the
effects on the bacterial microflora can be described as shown below.
The categorisation follows a recommendation drafted by the former Federal Institute for
Consumer Protection and Veterinary Medicine (BgVV, 2000), (now the Federal Institute for
Risk Assessment, BfR). This general approach has been adapted for the present purpose and
simplified.
The categorisation takes into account the treatment by the manufacturer (e.g. heat treatment,
other stabilizing procedures, use of preservation agents, fermentation), the possibility of
recontamination after this treatment and the type of packaging used. The recommended shelflife or best-before date are considered as well. The intended use at consumer level plays an
important role. For instance, consumption without further heat treatment in the kitchen, and the
consumption of specialised products by defined groups of consumers (e.g. diet or infant food).
The food matrix and characteristics also have a major influence on the bacterial microflora.
This concerns both intrinsic and extrinsic factors, including pH-value, NaCl-content, aw-value,
redox potential, temperature, storage conditions, etc.).
Some categories are only of importance for bacteria capable of multiplying in the food matrix
(e.g. Salmonella, Listeria). For bacteria that are unable to multiply (e.g. Campylobacter) in such
matrices, the nature of the food is not of importance. Bacteria introduced from the pre-harvest
13
EFSA Article 36 funded research project CFP/EFSA/DATEX/2007/02
14
ISO 16140 in revision by TC34 SC9 WG3
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Foodborne Antimicrobial Resistance
and harvest phases of the food chain pose a different risk to that posed by bacteria intentionally
introduced during processing.
Table 1 presents a categorisation of food for the purpose of undertaking an initial consideration
of issues relating to AMR. Notional sub-categories of the main categories are listed so as to
introduce technological factors as well as production factors for consideration. Formal subcategorisation of food groups would require to be based on such factors as the log reduction of
the bacterial load of concern brought about by the particular process used, and other
considerations. For the purposes of this Opinion any assessment based upon the sub-categories
as presented in Table 1 is qualified due to a lack of precision regarding the impact of the
specific process used on the particular food product’s microflora.
Any assignment of foods to the different AMR categories listed in Table 1 above is highly
subjective. Some foods may belong to two or more categories depending on the consumption
habits in different Member States. A simplified list is used here only to illustrate the different
categories and to provide a basis for a quantitative comparison of the relative contribution each
makes to the transmission of AMR bacteria to humans. Cross-contamination with these bacteria
at different stages of the food production chain (especially at retail level and in the home)
would affect the level of risk posed by such food irrespective of its category and would in effect
lead to a higher cumulative exposure than would be expected from the original food category
alone.
5.1.
Source attribution
In order to reduce the public health burden from foodborne infections (including that which
results from antimicrobial-resistant bacteria), it is important to have an insight into the source(s)
from which such bacteria gain entry to the food of concern. However this is not an easy
exercise because (1) many bacteria have multiple hosts, (2) there can be a vast range of
foodstuffs derived from one type of food-producing animal, and (3) humans may have
exposures to more than one possible source. Techniques developed for source attribution are
based on (a) outbreaks; (b) analytical epidemiology of sporadic cases (e.g. case-control studies);
(c) microbial sub-typing; (d) comparative exposure assessment and (e) expert opinion (Batz et
al., 2005). EFSA reports on methods for source attribution for human illness from foodborne
microbiological hazards (EFSA, 2008c), and source attribution for human salmonellosis from
meat (EFSA, 2008b), considers each of these in detail. Outbreak investigations, case-control
studies and microbial sub-typing studies have most commonly been applied to the area of
antimicrobial-resistant bacteria. For foodborne attribution, most attention has been centred on
Campylobacter and Salmonella (see sections 4.1.1 and 4.1.3). A source attribution analysis,
including antimicrobial-resistant Salmonella, is conducted annually in Denmark (Hald et al.,
2007).
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Foodborne Antimicrobial Resistance
Table 1.
An example of categorisation of food including production and processing
factors to facilitate the assessment of exposure of the consumer to AMR
factors.
Category concerning AMR (AMR Category)
Category and Subcategory of food
1.
Milk and dairy products (cows, goats sheep, buffalo, horse)
1.1. Milk
1.2. Dairy products (other than cheeses)
1.3. Cheese
2. Eggs and egg products
3.
Red meats
3.1. Bovine meat and products thereof
3.2. Pig meat and products thereof
3.3. Sheep meat and products thereof
3.4. Other or mixed red meat and products thereof
4.
Poultry meats
4.1. Broiler meat (Gallus gallus) and products thereof
4.2. Turkey meat and products thereof
4.3. Other or unspecified poultry meat and products thereof
5.
Aquaculture and marine
5.1. Fish and fish products
5.2. Crustaceans, shellfish, molluscs and products thereof
6.
Vegetables, cereals, fruits
6.1. Vegetables and juices and other products thereof
6.2. Cereal products including rice and seeds/pulses (nuts, almonds)
6.3. Fruit, berries and juices and other products thereof
7. Herbs and spices
8. Mixed or buffet meals*
9. Other foods*
10. Tap water including well-water
* Assessed by considering the food component subjected to the least amount of heat treatment or exposure to
comparable treatment, e.g. raw meat, raw vegetable, smoked fish.
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6.
On assessing the risk of the acquisition of antimicrobial resistant bacteria or
bacteria-borne antimicrobial resistance genes via the food chain
In accordance with the Terms of Reference, a reliable approach for assessing the risk to humans
of acquiring antimicrobial resistant bacteria or bacteria-borne antimicrobial resistance genes
from food is required. This is a complex task, as there are many possible routes of acquisition,
in addition to food, such as direct contact with livestock and companion animals, exposure to
the environment, human-to-human transmission, etc. Here we focus only on the food routes.
Human exposure to antimicrobial resistant bacteria is difficult to measure (qualitatively or
quantitatively). Data on the quantitative numbers of antimicrobial resistant bacteria in different
food products and data on the human consumption habits are in some cases available but may
not be in the required format for input into a risk assessment. It is unknown whether
antimicrobial resistant bacteria survive or multiply during stages of the food-chain (e.g.
processing, cooking etc.) to a greater extent than susceptible bacteria. Likewise, in terms of the
dose-response characteristics, there are very limited data on whether resistant bacteria are more
pathogenic or cause more severe illness than the antimicrobial-susceptible equivalent. In
addition, it is very difficult and the data very sparse, to properly take into account the
significance of transferable resistance genes and their ‘indirect’ impact on human health. Few if
any risk assessments in this area have considered this consequence, presumably due to the
significant data requirements and, overall, the scientific uncertainty associated with within-host
resistance gene transfer.
It is recognised that there are many different types of consumers and that their consumption
habits (e.g. type and quantity of food consumed) and susceptibility to antimicrobial resistant
infections may differ. For example, the ‘consumer’ can be classified as an infant, youth, adult
or an elderly person and within each of these categories, could be further classified as healthy,
clinically ill or immuno-compromised. In the ideal world, a risk assessment would also take
into account a secondary classification to reflect cultural and religious status and optional
dietary preferences (vegetarians, vegans). Likewise, taking into account the risk of exposure,
farming families and workers, along with workers in the meat trade deserve consideration as
distinct entities as, either usually or occasionally, they may consume raw dairy and meat
products. Other groups engaged in the wholesale or retail food trade may be similarly exposed.
Many types of consumers are identified here and we acknowledge the potential impact of each
type on their risk of exposure and any consequences, due to the large scope of the given Terms
of Reference, consideration of consumer type is not taken any further here.
6.1.
Issues to be considered in relation to risk assessment applied to the area of
antimicrobial resistance
Risk assessment is a scientific tool that can be used to evaluate the level of exposure and the
subsequent risk to human health due to a specific microorganism or particular type of
resistance. Both qualitative and quantitative risk assessment approaches have been utilised to
estimate the risk to human health from antimicrobial resistant bacteria (Snary et al., 2004).
Written guidelines and accepted procedures are available (e.g. Codex Alimentarius
Commission, 1999) for microbial food safety risk assessments and for antimicrobial resistance.
The OIE guidelines, which are specific to antimicrobial resistance risk assessment, can also be
used (OIE, 2007a). Risk assessments in the area of antimicrobial resistance, and especially
those investigating the impact of the use of antimicrobial agents in food animal production on
human health, are challenging. This is because the data needs are greater than for non-resistance
risk assessments and for many aspects there are significant data gaps.
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Foodborne Antimicrobial Resistance
6.1.1.
Data requirements for an antimicrobial resistance risk assessment
The data requirements will be determined by the risk analysis question posed and the level of
detail (or resolution) used to address this question. There is no standard list; however, previous
data gaps/deficiencies were identified by Snary et al., (2004) and are summarised in Table 2.
Here some of the data requirements (and gaps/deficiencies) and hence the challenges
encountered in the area of antimicrobial resistance risk assessment, are discussed, but are
limited to risk assessments that focus on transmission of antimicrobial-resistant bacteria
through the food chain.
If the focus of the risk assessment is on the use of a certain antimicrobial in food-animal
production it is often the case that data on the usage of antimicrobial agents for food animal
species are in many Member States totally lacking. If such data are available, it is very rarely, if
ever, known down to the individual animal, herd or flock level. The exact association between
usage of a given antimicrobial agent and the emergence and spread of resistance is seldom
known and even though several studies have shown that usage is an important factor for the
emergence of resistance, the association is not linear, but is also determined by the way the
antimicrobial agent is used. Thus, on the one hand it has been indicated that increased dosages
might help to avoid the selection for quinolone resistance in Salmonella (Wiuff et al., 2003),
while on the other hand, continuous feeding of tylosin supplemented feed to chickens might
select for macrolide resistant C. jejuni, whereas single treatments are less likely to do so (Lin et
al., 2007).
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Foodborne Antimicrobial Resistance
Table 2.
Key data limitations/issues affecting microbial risk assessments (MRAs)
applied to the area of antimicrobial resistance (Snary et al., 2004)
Data limitation/issue
Effect on MRA
Definition of resistance
•
Data from different sources are not
comparable. May limit the amount of data
available for the MRA.
•
The amount of data available for the MRA
may be limited if the methods are not
comparable.
•
Cannot compare selective plating against the
testing of one isolate without knowledge of
the ratio of resistant to susceptible bacteria.
•
If enriched the number of organisms is
increased and therefore cannot directly be
used in the MRA.
Multiple levels of the sampling framework
•
Large variability of sampling methods
between studies. Therefore data from
different sources may not be comparable;
could limit the amount of data available for
the MRA.
Small sample sizes
•
If the sample size is small at any level of the
sampling framework, the uncertainty about
the associated parameter will be large. This
may contribute to a large uncertainty
associated with the final risk estimate.
Little data available on indicator organisms
(resistant or susceptible) compared to pathogenic
bacteria.
•
Surrogate organisms etc. may be used to
overcome the data gap, thus increasing the
level of uncertainty in the output of the
model. This uncertainty may not be
quantified.
Sensitivity and specificity of the tests used.
•
MRA may overestimate or underestimate the
risk.
Causality unclear
•
Large assumptions made on the causality of
antimicrobial resistance. This leads to a
higher level of uncertainty in the model
results, but which may be difficult to
quantify.
Lack of quantitative microbiological data
•
Microbial load of resistant bacteria in/on
different sources is unknown, therefore either
not modelled or key assumptions made.
Little information on the use of antimicrobial
agents for
•
Causality is difficult to consider. May lead to
a large degree of uncertainty in the results of
the model.
−
Harmonization of MIC/disc-diffusion
breakpoints required.
Microbiological methods, e.g.
−
Selective plating v testing of one isolate from
non-selective plate
−
Enrichment v non-enrichment
−
Molecular versus phenotypic methods
−
veterinary use (at animal and farm level)
−
human use
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6.1.2.
Requirements for a risk assessment
It is very difficult to provide a general definition for a risk assessment. This is because the most
important attribute is that it is ‘fit for purpose’, i.e. it answers the risk question posed within the
constraints of the resources available (e.g. time, data and expertise).
As described in the Terms of Reference, the aim here is (1) to identify in terms of qualitative
risk, the extent to which food serves as a source for the acquisition, by humans of antimicrobial
resistant bacteria or bacteria-borne antimicrobial resistance genes; (2) to rank the identified
risks and (3) to identify potential control options for reducing exposure. Therefore, in the ideal
world, for the Terms of Reference given, all factors that increase/decrease the risk of human
exposure (both in terms of prevalence and microbial load) to a particular antimicrobial-resistant
bacteria from a particular source would be considered as part of the risk assessment and the
required data would be available. In particular, the food pathways would take the form of a
farm-to-consumption risk assessment and would be able to take into account the variability of
production systems and consumer preferences between the different EU Member States. In
addition, as discussed earlier, detailed risk assessments would be produced for the other sources
of antimicrobial-resistant bacteria and would need to take into account the different exposures
and consequences that sub-populations of consumers may have. In addition to exposure
assessment, a full risk assessment would also need to take into account the dose-response
relationship of developing infection and clinical illness. Specific for AMR risk assessment, the
consequences of resistance on outcome of infection and illness (e.g. treatment failure), would
need to be included. Finally, the problem of within-host (human) resistance gene transfer would
need to be taken into account to ensure that the risks of ‘direct’ and ‘indirect’ transmission are
comparable. This would be difficult if using the probability of exposure as the end-point of the
risk assessment were used.
Developing a risk assessment along the lines described above would allow the risks to be
estimated for each possible source and hence ranked. In addition, due to the detail included in
the risk pathways, many control measures (individually or simultaneously) could be
investigated and their effect on the risk and ranking assessed. However, to do this in full,
would be extremely challenging and would probably take multiple person-years. This is
especially due to the number of antimicrobial classes that would need to be considered (see
Appendix: Table A), the bacteria of interest (Salmonella, Campylobacter, VTEC,
Staphylococcus aureus, etc) and the number of potential sources, where the food routes alone
account for 20 different categories (Table 1) without, however, taking into account the precise
degree of processing (e.g. raw, minimally processed and processed).
For the above reasons the assessment presented here for illustrative purposes only, is an
assessment of the risk of exposure to AMR bacteria where food is the vehicle of interest. While
the assessment is designed to be qualitative, this is nevertheless a large and complex risk
question. Consequently, a simplified approach to assessing the extent to which food serves as a
source is preferred here. This approach allows the food types to be compared and hence ranked
for a particular antimicrobial-resistant bacterium. There is no intention to propose a method
whereby specific bacterial species/antimicrobial resistance combinations could be prioritised.
Due to the simplicity of the approach, the template is not amenable, as more complex risk
assessments would be, in terms of assessing the effect of control options. Neither is this
approach put forward as a means of addressing such issues as emerging risks.
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Foodborne Antimicrobial Resistance
6.2.
Construction of an exposure assessment template: Food as a source of
antimicrobial resistant bacteria. An example.
6.2.1.
Exposure pathway
Rather than adopting a farm-to-fork approach, in this example, the risk pathway commences at
the point of retail sale (Figure 2). This removes the need to include the earlier production
stages of farm, transport and lairage, abattoir and further processing. In addition, it is closer to
the point of consumption of a food-stuff and, advantageously, many Member States collect
information on the prevalence of bacteria and also antimicrobial resistance at the point of retail.
Even though the pathway does not implicitly take into account undercooking of food products
or cross-contamination the prevalence of the antimicrobial-resistant bacteria at the point of sale
is used as a proxy to indicate the degree of contamination that is entering the home/restaurant.
Contamination that may occur following purchase is not considered in this example. The
probability of bacteria being present in food at retail and the probability that bacteria present in
food at retail are resistant to an antimicrobial class of interest can be combined,
multiplicatively, to provide an overall probability of the food at retail being contaminated with
antimicrobial-resistant bacteria. This is combined with the probability that the food is
purchased and consumed; such data should be available from consumption studies (e.g.
Harrington et al., 2001). Each of the data requirements for the proposed risk pathway are
considered below. The preferred end-point of the risk pathway would be the probability of a
human being exposed to the antimicrobial -resistant bacteria of interest due to the consumption
of the food of interest. Because data on cross-contamination and the effect of food preparation
practices on the viability of AMR bacteria are scarce, as well as dose-response and consequence
data, the exposure assessment, in this example, stops at the point of purchase of food at retail.
Existing data on cross-contamination involving non-AMR bacteria could be substituted,
however, as an extension to the present study.
The hazard characterization phase of the complete risk assessment process (e.g. dose-response;
severity of illness; treatment failure, etc.) is not considered here. Given the end-point of
exposure, this template can also be used for indicator bacteria that carry resistance genes.
However it is essential that the interpretation of the final results takes into account the
differences in the hazards. This applies, in particular, when comparing the more ‘direct’
transmission of resistant foodborne pathogens (e.g. macrolide-resistant Campylobacter;
fluoroquinolone-resistant Salmonella) to the more ‘indirect’ risk from indicator bacteria (e.g.
ESBL-resistant E. coli and vancomycin-resistant Ent. faecium) and also the indirect risk posed
by pathogens carrying readily transferable resistance genes (e.g. Salmonella carrying plasmid
borne ESBL resistance) where gene transfer within the human gut needs to be considered as
part of the discussion. The same would apply to bacteria that are intentionally added to foods,
such as fermentation bacteria. A full assessment of the effect of exposure to horizontally spread
genes would be extremely complex and require data that are not readily available.
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Foodborne Antimicrobial Resistance
Probability
of
bacteria
being
present in food at
retail
Probability that bacteria
present in food at retail
is
resistant
to
antimicrobial class of
interest
(MULTIPLICATION)
Probability of food at
retail being contaminated
with AMR bacteria
Probability that food is
purchased and consumed
Probability of
AMR
bacteria in components of
a food before preparation
Figure 2.
Example of a risk pathway for assessing the contribution of different foods to
the occurrence of AMR bacteria in meal components.
Finally, it should be noted that although the adoption of a simplified approach such as this
makes the risk ranking much more feasible, it loses resolution in terms of being able to
explicitly consider the impact of control measures on the risk ranking. Consequently, unless
information is gained on the effect of interventions on any of the 3 model parameters, namely
the probability that (i) the bacteria in question are present in food at retail; (ii) such bacteria are
resistant to the antimicrobial class of interest; (iii) the food is purchased and consumed, it will
not be possible to assess the impact of control measures on the risk ranking. Therefore the
identified potential control options for reducing exposure may not be included within the risk
assessment framework, but by using other relevant evidence (e.g. epidemiological studies) can
be used to support the recommendation of such control options.
6.2.2.
Data requirements and availability
For each of the data requirements in the risk pathway, an estimate by category is provided,
either using available data or expert opinion. In order to allow transparency and consistency
between food-types and other sources, the categories are defined by broad ranges of
probabilities. The number of categories is limited to three or four, because the presently
available data do not justify more precise categories.
The EFSA Journal (2008) 765, 41-87
Foodborne Antimicrobial Resistance
6.2.2.1. Probability of bacteria being present in food at retail
At a national level, data are likely to be available for the probability of the bacteria of interest
being present in food at retail (i.e. prevalence). However, in practice, data quality and quantity
will vary between Member States (MS). For example, some MS may have carried out large,
structured, retail surveys and others carried out smaller studies where the sampling was done by
convenience rather than randomised. In addition, the microbiological methods may differ
between studies and between food types. As for all the probabilities being considered,
significant variation between MS and even regions within MS may be expected.
6.2.2.2. Probability that bacteria present in food at retail are resistant to antimicrobial class of
interest
Antimicrobial resistance testing can also vary between countries (and will have the same study
design issues as identified above). Many studies pick a single colony of the bacteria and test
this for antimicrobial resistance using a non-selective culture plate; other studies put the culture
substrate onto primary isolation media containing an antimicrobial. Depending on the ratio of
resistant to susceptible bacteria in the sample, this may affect the estimated probability of the
antimicrobial-bacteria being present in the food and may make it difficult to compare studies
and hence the different food sources.
6.2.2.3. Probability of AMR bacteria in food at retail
This probability is simply a multiplication of the two probabilities discussed above. Three
categories are distinguished (high, >1%; medium, 0.01 - 1 %; low, <0.01%)
6.2.2.4. Probability that food is purchased and prepared for consumption
The probability of the food of interest being purchased and consumed can be obtained from
national consumption studies. Such studies vary in the level of detail of the different food stuffs
consumed and also the desired output from such studies, as many are designed for nutritional
rather than food-safety purposes. The food categories suggested in Section 5 are extensive in
number, but are still a simplification of the diverse range of foods that Europeans eat. For each
food stuff, where appropriate, different levels of processing are taken into account as this will
affect the risk of the consumer being exposed to the hazard of interest. However, it may not be
possible to break down the consumption data to, for example, the level of raw, minimally
processed and processed. Consequently, if not available, this must be done using expert opinion
and hence bringing further uncertainty into the assessment. Four categories are detected, which
characterise the proportion of consumers who would eat a meal including the food of concern
on a random day.
6.2.3.
Presenting the risk estimate
In this preliminary risk assessment, the risk of preparing a meal with food components that are
contaminated with AMR bacteria is simply presented by cross-tabulation. This eliminates the
need to apply seemingly simple, but arbitrary combinatorial rules.
6.2.4.
Case-study 1: Fluoroquinolone-resistant Campylobacter jejuni in the UK
The framework described above is now adopted for a risk assessment for fluoroquinoloneresistant C. jejuni in the UK. For each food-stuff, information is obtained for the 3 parameters
The EFSA Journal (2008) 765, 42-87
Foodborne Antimicrobial Resistance
listed above, i.e. probability of bacteria being present in food at retail; probability that bacteria
present in food at retail is resistant to antimicrobial class of interest and the probability food
purchased and consumed. Table C in the Appendix provides the information that was collected
and the outcome of the assessment. It is important to note that the data collection was not
exhaustive and that the data included is what was readily available to the working group at the
time. Consequently, it has been necessary to make many assumptions when constructing Table
C. It is therefore essential to note that this is not a formal risk assessment but, rather, an
example of how to complete the template and the type of information that would be
informative. Taking this approach, broiler meat that is bought raw is expected to have the
highest probability of carrying fluoroquinolone-resistant C. jejuni. Other products with
relatively high risk are raw beef and pork. Of course, in the majority of cases, these products
will be cooked but, as described before, using this output provides a measure of the degree of
contamination that is entering the home/restaurant. Note that raw vegetables, fruit etc., and also
certain beef products are typically consumed without further cooking; in these cases the relative
risk of consumer exposure would actually be higher than suggested in this Table.
The completion of the template for just one combination of bacteria, antimicrobial and country
demonstrates the size of the task requested by the TOR. In particular, the data collection phase
would be significant. As seen in Table C, data for the more common food sources of the
bacteria will be plentiful, but not for those that are deemed to be more unusual. The same
applies for the antimicrobial resistance data, where it is frequently assumed that the probability
of Campylobacter being fluoroquinolone-resistant in minimally processed and processed foods
is the same as in fresh/raw food stuffs. Such a probability is based upon the implicit assumption
that any decay of fluoroquinolone-resistant C. jejuni during processing happens at the same rate
as for other Campylobacter spp. Care must also be taken when comparing antimicrobial
resistance data as different break-points may have been used, e.g. the majority of data referred
to use a break-point of 16 mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin; however
the study on raw/fresh broilers by Wilson (2003) used a breakpoint of 30 mg/litre for nalidixic
acid. Small sample sizes are also an issue. In quantitative risk assessment, the uncertainty can
be described, often using a Beta distribution, but this is not possible using a qualitative risk
assessment approach. In Table C, when sample sizes have been low the working group has
erred on the side of caution and/or made assumptions.
Detailed consumption data can also be difficult to obtain. Using the Irish data (Harrington et
al., 2001), although there was good information on each type of food, there was no information
on the level of processing for each food-type at the point of retail, i.e. whether the food
consumed was purchased at retail as fresh/raw, minimally processed or processed.
Consequently many assumptions had to be made, thereby adding to the uncertainty associated
with the individual risk estimates. For some of the food types, there was no information
available, or if there was information, the sample size was very small, e.g. in the case of
minimally processed fruit, berries and juices. These limitations should be considered when
comparing this source of fluoroquinolone-resistant C. jejuni to other food-types.
The EFSA Journal (2008) 765, 43-87
Foodborne Antimicrobial Resistance
Table 3.
Examples of the risk of purchasing food contaminated with fluoroquinoloneresistant Campylobacter
(Prevalence data from UK (see Table C in the appendix), “purchasing” data from
Prevalence
of
FQresistant Campylobacter
Frequency of consumption of purchased food items
Daily (>50%)
Weekly (5-50%)
Monthly (0.5-5%)
Rarely (<0.5%)
High (>1%)
Raw broiler meat
Medium (0.01-1%)
Raw beef
Raw pork
Raw sheep
Raw turkey
Offal
Private water supplies
Raw milk
Raw dairy
Low (<0.01%)
Processed milk
Processed dairy
Processed cheese
Eggs
Fish
Vegetables
Soft fruit
Juices
Cereals
Community water supplies
Processed beef
Processed pork
Processed sheep
Processed poultry
Raw shellfish
Game
Raw cheese
6.2.5.
Future development of risk assessment approaches
As has been indicated before, full risk assessments of AMR bacteria in foods are demanding in
terms of data availability and resources. This is not a characteristic of the risk assessment as
such, but rather of the risk management questions. Comparing the risks of different pathogens
in different foods is a demanding task that cannot be done by any approach without adequate
resources. Likewise, the impact of potential control options at some stage in the production
chain on the risk of consumer exposure and/or health is a complex issue.
A possible strategy is to build up AMR risk assessments on the basis of available risk
assessments for sensitive bacteria.
For the purpose or risk ranking, an exposure assessment model as presented by Evers et al.
(2008) could be adopted. This model, which is also discussed in the EFSA Opinion on
Salmonella in meat (EFSA, 2008b), estimates exposure per person per day, averaged over a
specified population (e.g. all inhabitants of one country). Exposure is estimated separately for
all relevant sources (different food products, but also animal contact, environment, etc.). For
food sources, the average exposure is estimated by multiplication of (averages of) the daily
intake of the food product, the fraction of contaminated products at retail, the concentration of
pathogens in contaminated products at retail and the fraction of pathogens that is eventually
ingested by consumers. For foods that are consumed raw, this fraction is 1; for foods that are
cooked before consumption the fraction is between 0 and 1 as this fraction can result from
undercooking and/or cross-contamination. Similar factors are taken into account for
environmental (e.g. water) exposure. For animal contact, in the course of food preparation,
calculations involve factors such as the frequency of human-animal contact and the (probability
of) ingestion of faeces per contact.
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Foodborne Antimicrobial Resistance
Results of all exposures can be cumulated to calculate the total exposure or can be ranked to
identify the most significant sources of exposure. There are currently many data gaps, and
uncertainty analysis is an essential component of the calculations. Uncertainty is explicitly
included in the exposure estimates. For AMR risk assessment, additional data are necessary on
the prevalence of resistant bacteria in all exposure routes to be considered. Such data are
available from the literature, from special studies or by using proxies (e.g. the prevalence of
AMR bacteria in raw milk is similar to that in cattle faeces).
The exposure assessment model can be regarded as an extension to the cross-tabulation
approach presented in this document. The exposure model takes the same variables into account
but is based on quantitative rather than categorical estimates. Furthermore, it also includes the
effects of preparation and cross-contamination.
Risk assessment models that need to evaluate the effect of interventions on AMR risk can also
be built on existing (farm-to-fork) models. For example, EFSA has currently outsourced a
QMRA on Salmonella in pigs15. This model can in future be simply extended to include the
spread of resistant salmonellae in the food chain by multiplying the prevalence of Salmonella at
the farm gate by the percentage of bacteria examined that are resistant. The underlying
assumption would be that the behaviour of resistant bacteria in the food chain is similar to that
of sensitive bacteria of the same genus, species or serotype. In the absence of selective pressure,
this appears to be a realistic assumption. A more complex question would be to evaluate, inter
alia, the impact of a reduced use of antibacterial agents in primary production. This would be
subject to the development of new modules on the relationship between usage of and resistance
to antimicrobials.
6.2.6.
Antimicrobial resistance genes in genetically modified organisms
For GM plants, which can be present in food:
While this opinion primarily deals with AMR bacteria in foods, concerns have been raised
about the possible link between the presence of antibiotic resistance marker genes in GM plants
and the increase of resistance against relevant antibiotics in human, animals and in organisms in
the wider environment as a result of horizontal gene transfer. The GMO Panel in its opinions
concludes that this route of antibiotic resistance development is extremely unlikely. The
conclusion is based on the fact that the successful transfer of a functional antibiotic resistance
gene (or any other gene) from a GM plant into a bacterium would require a series of
biologically complex and unlikely events to occur (EFSA 2004b and EFSA 200716).
The use of antibiotic resistance marker genes in GM plants has been the subject of several
reviews (Gay and Gillespie, 2005, Goldstein et al., 2005, Miki and McHugh, 2004, Nap et al.,
1992, Nielsen et al., 1998, Ramessar et al., 2007) and expert consultations: Working Party of
the British Society for Antimicrobial Chemotherapy (Bennett et al., 2004), FAO/WHO
Consultation on Foods Derived from Biotechnology (FAO/WHO, 2000), Scientific Steering
Committee of the European Commission (SSC, 1999) Zentrale Kommission für die
Biologische Sicherheit, DE (ZKBS, 1999), The Advisory Committee on Novel Foods and
Processes, UK (ACNFP, 1996). It has been concluded in these reports that the frequencies of
gene transfer from plants to bacteria are likely to be extremely low and that the presence of
15
EFSA Article 36 Cooperation, call for proposal, CFP/EFSA/BIOHAZ/2007/01: Quantitative microbiological risk
assessment
on
Salmonella
in
slaughter
and
breeder
pigs.
www.efsa.europa.eu/EFSA/efsa_locale1178620753812_1178622332966.htm
16
www.efsa.europa.eu/EFSA/Statement/gmo_statement_nptII_,0.pdf
The EFSA Journal (2008) 765, 45-87
Foodborne Antimicrobial Resistance
antibiotic resistance marker genes in GM plants do not pose a relevant risk to human or animal
health or to the environment.
7.
Prevention and control options
Proposals for the control of the transmission of AMR bacteria and resistance genes to humans
through the agency of food require to take account of the factors that give rise to AMR and to
the ways in which food becomes exposed to contamination with these agents (Figure 1).
Regarding the former, since the use of antimicrobials in human and veterinary medicine is the
major initiating factor for such resistance, the control and conditions of use of antimicrobials in
both fields have been extensively addressed elsewhere and are the subject of various reports
(WHO, 2000, 2001; Codex, 2005). The induction of AMR through the therapeutic use of
antimicrobials in human and veterinary medicine is an inevitable consequence of the ethical
need, on health and welfare grounds, to use such treatments in a clinical situation. Of particular
concern is the impact of their continued use in the form of mass medication for the treatment of
infectious diseases in food animals kept in intensive production systems. This issue has been
comprehensibly addressed elsewhere (WHO, 1997, 2000).
The dissemination of bacteria that have acquired AMR attributable to human medical
treatment, both in a hospital setting and in the home, occurs in both the general environment
and in the home. When this occurs in the environment of the kitchen, then food becomes
exposed as the result of direct or indirect contamination, e.g. through handling. Consequently,
the prevention and control of food contamination with antimicrobial-resistant bacteria, both
pathogenic and otherwise, from this and other sources, relies on the consistent and effective
application of good food hygiene practices. Of equal if not greater importance is the prevention
and control of the spread of AMR bacteria originating from primary food animal production
and to a lesser extent from contamination in the course of harvesting, processing and
distribution. Here again the sustained application of good hygienic practices (Council Directive
93/43/EEC) throughout the food chain provides a varying degree of assurance against the
introduction of AMR bacteria onto or into food, as has been adequately demonstrated in the
case of known pathogens and the control of spoilage bacteria.
Recently, other concerns have arisen in relation to bacterial contaminants of processed foods in
which AMR has resulted from transformation induced by the effects of modern processing or
preservation methods, and the possibility that the increasing use of biocides in industry and in
the home may itself induce AMR in a wide range of bacteria. The dissemination of such AMR
bacteria, were they to arise, would likely be addressed through the application of good hygienic
practices or, where necessary, by modification or suspension of the food processing involved
and by the selective use, or the withdrawal from use, of biocides shown to induce AMR. In
industry the dissemination of those AMR microorganisms can be mitigated by using proper and
convenient validated physical treatments (for example, sterilization or pasteurization
treatments).
Further control options that address the induction of AMR in bacteria and that are aimed at
limiting the spread of such bacteria are discussed below.
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Foodborne Antimicrobial Resistance
7.1.
Controlling spread of infections and of resistant bacteria
7.1.1.
Preventing infectious diseases in animals and plants
Reduction of animal diseases can be expected to reduce the need to use antimicrobials in food
production. Measures to reduce disease in animals include specific measures such as
vaccination and the prevention of spread through biosecurity and general operational hygiene
management measures.
The use of antimicrobials for treatments against plant pathogenic bacteria is generally not
permitted in European countries, although the situation varies between MS (McManus et al.,
2002). However, in other parts of the world where antimicrobials are registered for use against
the fire blight of Rosaceae, widespread resistance to streptomycin has been reported for Erwinia
amylovora, the causal agent of fire blight (McManus et al., 2002).
Measures which may help in reducing the inoculum and the spread of bacterial disease in plants
are the use of healthy pathogen-free plant propogation material and resistant plant varieties, the
application of protective treatments with copper compounds and the adoption of correct cultural
hygiene practices.
7.1.2.
Control and prevention of Salmonella and other zoonotic bacteria in animals
The use of programmes aimed at the prevention and control of Salmonella and other zoonotic
bacteria in primary animal production, can lead to a reduction in the level of contamination of
related food products at retail, and thereby also reduce the risk of human exposure to AMR
salmonellae from those food products. The occurrence of Salmonella and AMR salmonellae in
other food commodities is also likely to be reduced as the risk of cross-contamination is
reduced.
In all cases, antimicrobials have no part to play in control programs for Salmonella in food
production (e.g. EFSA, 2004a, 2006c).
7.1.3.
Improved hygiene
Improved hygiene at all steps of the food chain, including primary production, is effective in
reducing the number of foodborne pathogens in food. This will also reduce the numbers of
foodborne pathogens that are resistant to antimicrobials.
7.1.4.
Processing
Most food processing technologies aim to reduce the level of contamination of foods with
bacterial pathogens as well as the overall bacterial load. As a consequence, the presence of
foodborne AMR bacteria is also reduced. In addition, bacteria added intentionally to the food
chain may also contribute to the control of foodborne pathogens,. they should however be free
of potentially transferable antimicrobial resistance before their application in feed or food
processing.
7.1.5.
Recirculation
Animal manures and municipal sludges, particularly in the latter case those sludges that contain
effluents from hospitals, contain many types and numbers of pathogenic and other bacteria,
The EFSA Journal (2008) 765, 47-87
Foodborne Antimicrobial Resistance
including AMR bacteria in both these categories. Hospital effluent has been demonstrated to
contain a high proportion of AMR E. coli (Chitnis et al., 2000; Reinthaler et al., 2003) and
vancomycin resistant enterococci on occasion (Iversen et al., 2002). This is not to discount the
contribution of AMR bacteria contributed by the effluent from the general population.
The WHO has indicated that in countries that do not experience epidemics of enteric disease, it
is acceptable to discharge the effluent from health-care establishments to municipal sewers
without pretreatment, provided specific requirements are met (WHO, 1999). If these
requirements cannot be met, the wastewater should be managed and treated accordingly.
Proper management of both these materials, if their application on land used for food
production or their discharge into waterways and estuaries serving aquaculture is intended, can
effectively address the risk they pose for food animals and fresh produce produced on these
lands and in these waterways. Any consequential transmission onto food of AMR bacteria and
genes derived from animal manures and municipal sludges can be controlled concurrently by
employing processes used for the treatment of manures and municipal sludge that effectively
mitigate any food-related risks to human health posed by such use.
7.2.
Appropriate usage of antimicrobials
Reduction of the use of antimicrobials in general, or of specific antimicrobial classes, reduces
the selective pressure and in many cases will thereby reduce the prevalence of resistant bacteria.
A reduction of use can be obtained in different ways as detailed in, e.g. the SSC report (1999),
the OIE guidelines for the responsible and prudent use of antimicrobial agents in veterinary
medicine (OIE, 2007a), WHO Global principles for the containment of antimicrobial resistance
in animals intended for food (WHO, 2000) and the WHO global strategy on containment of
antimicrobial resistance (WHO, 2001). For example, a drastic reduction in their use may be
encouraged through regulatory interventions, such as withdrawal of authorization or other
restrictions. However, antimicrobials are needed to treat animal diseases and therefore, these
measures can only be applied where such use is unnecessary or where there are clear
alternatives available.
A sharing of responsibility on the part of all stakeholders, i.e. advisers, producers, processors,
distributors and those involved in final stages of food preparation, that is based on a knowledge
and appreciation both of the consequences of AMR for the human patient and the means of
retaining an effective arsenal of antimicrobial agents, is recognised as a key factor when
addressing AMR as a global issue of grave concern. Measuring the effectiveness of
interventions and identifying priority areas
Monitoring of the occurrence of antimicrobial resistance, as well as the extent of use of
antimicrobials and their use in human medicine and food animal production can provide
relevant background information when considering trends in antimicrobial resistance and its
prevalence in relevant bacteria, including pathogens and non-pathogens, in foods. This
information can provide a further means to identify problems, to measure the effect of
interventions and to support policies on the use of antimicrobials.
8.
Issues of immediate concern
Fluoroquinolone antimicrobials are an important addition to the list of antimicrobials available
for the treatment of infectious diseases. The appearance and spread of strains of enterobacterial
pathogens such as Salmonella Typhi, Typhimurium and Enteritidis with reduced sensitivity to
The EFSA Journal (2008) 765, 48-87
Foodborne Antimicrobial Resistance
ciprofloxacin coupled with high-level resistance to nalidixic acid has been described in sections
4.1.1. and 4.1.2. above. A new development has been the emergence of strains with plasmidmediated fluoroquinolone resistance in several countries world-wide, in both humans and foodproduction animals. Such plasmid-mediated resistance has resulted in an increased MIC to
ciprofloxacin, with adverse effects for treatment (Hopkins et al., 2008). Strains with such
resistance are rapidly increasing in incidence, and may pose a significant threat to public health.
The potential role of food and environmental sources in the epidemiology of transferable
resistance genes has gained increased attention in relation to the rapid and recent emergence of
resistance to 3rd generation cephalosporins, in particular of the CTX-M-type (Canton and
Coque, 2006; Livermore et al., 2007). The genes coding for these enzymes may be located on
highly transferable plasmids and are found in bacteria causing infections in hospitals, but also
in infections acquired in the community, in Salmonella from cases of human infection and food
animals and commensal E. coli isolated from animals (Livermore et al., 2007). The genes
encoding this type of resistance may be physically linked in mobile genetic structures with
fluoroquinolone resistance, and also with genes encoding resistance to other resistance genes
(Canton and Coque, 2006). The role of food, water and the environment in the spread of
apparently epidemic plasmids encoding multiple resistance is not clear, but deserves immediate
attention.
Concerns regarding the increasing rate of isolation of MRSA from food producing animals and
whether or not there is a link to public health through food now need to be addressed.
In view of experimental findings, the possibility that new food processing and preservation
treatments may induce AMR in commensal and other bacteria, as a result of transformation,
merits attention.
In relation to food as a vehicle for their transmission to humans, other aspects of AMR and the
emergence of new patterns of resistance in bacteria that to-date have attracted little attention are
now likely to arise as a focus of concern due to changing patterns in medical and veterinary use
of antimicrobials, in food consumption and in international trade in food.
CONCLUSIONS AND RECOMMENDATIONS
CONCLUSIONS
•
The principles that are applied to the prevention and control of the spread of pathogenic
bacteria via food will also contribute to the prevention and control of the spread of
antimicrobial-resistant pathogenic bacteria. As antimicrobial resistance in foodborne
pathogens and commensals represents a specific public health hazard, additional control
measures for antimicrobial-resistant bacteria may therefore be necessary.
•
The present extent of exposure to AMR bacteria via food is difficult to determine and the
role of food in transfer of resistance genes has not been fully explored to-date. Any further
expansion of the occurrence of resistance among bacteria in foods, including fresh cropbased foods, is likely to have an influence on human exposure.
•
Foodborne bacteria, including known pathogens and commensal bacteria, display an
increasing, extensive and diverse range of resistance to antimicrobial agents of human and
veterinary importance.
The EFSA Journal (2008) 765, 49-87
Foodborne Antimicrobial Resistance
•
Antimicrobial resistance in food exists both as a direct hazard and as an indirect hazard
through resistance transfer.
-
The direct hazard is the presence on food of an AMR pathogenic bacterium which can
colonise or infect a human being after ingestion of the food, or as a hazard that arises if
a person acquires the infection through handling contaminated food.
-
The indirect hazard arises through resistance transfer and is defined as an antimicrobialresistant bacterium that may transfer resistance genes to another bacterium that is either
a commensal or a bacterium pathogenic for humans.
•
In all cases where antimicrobial treatment in humans is indicated, resistance to the
antimicrobials of choice is of clinical importance.
•
Resistant Salmonella and Campylobacter involved in human disease are mostly spread
through foods. With regards to Salmonella, contaminated poultry meat, eggs, pork and beef
are prominent in this regard. For Campylobacter, contaminated poultry meat is prominent.
•
Cattle are a major VTEC reservoir and resistant strains derived from bovines can colonise
the human population via contaminated foods of bovine origin more commonly than from
other foods.
•
Food is also an important source for human infections with antimicrobial resistant Shigella
spp. and Vibrio spp.
•
Animal-derived products remain a potential source of MRSA. Food-associated MRSA,
therefore, may be an emerging problem.
•
Bacteria intentionally added to the food chain have on occasion exhibited AMR. As such
they are to be regarded as an indirect foodborne hazard as in this case the hazard is
considered as being the resistance gene.
•
The public health consequences of exposure to antimicrobial-resistant commensal bacteria
through food are less well defined.
•
Recently identified links between AMR and virulence in foodborne pathogens are a cause
for concern. Any enhancement of virulence in known pathogenic bacteria, and potentially in
other bacteria as yet unidentified as pathogenic, as a consequence of acquiring resistance
attributable to antimicrobial usage or gene transfer can adversely affect the outcome of
treatment.
•
By way of example, a qualitative ranking of food as a vector of an AMR bacterium
demonstrated the complexity of the problem and the extensive data requirements for a
formal ranking of risk.
•
Any control measure requires to be viewed in the context of the critical and irreplaceable
role specific antimicrobial therapeutic agents or groups of agents play in the treatment and
management of life-threatening infectious diseases in humans.
•
There are few examples of control programmes that directly control AMR as the hazard
using measures that specifically address food, the final product, as the vehicle of concern. In
terms of impact, controls operated at the pre-harvest phase, for example those aimed at the
control and limitation of antimicrobial usage, are potentially the most effective and as such
are capable of playing a major role in determining the AMR-status of food as presented for
sale.
The EFSA Journal (2008) 765, 50-87
Foodborne Antimicrobial Resistance
RECOMMENDATIONS
The development and application of new approaches to the recognition and control of food as a
vehicle for AMR bacteria and related genes based on epidemiological and source attribution
studies directed towards fresh crop-based foods, raw poultry meat raw pigmeat and raw beef are
recommended.
The use of epidemiological cut-off values provides an appropriate level of sensitivity when
measuring resistance development in bacteria. These criteria have been harmonised for use in
both in human and veterinary medicine in the European Union. It is now important that these
matters be addressed globally.
Specific measures to counter the current and developing resistance of known pathogenic
bacteria to fluoroquinolones as well as to 3rd and 4th generation cephalosporins found in a
variety of foods and in animals in primary production now require to be defined and put in
place as a matter of priority.
As a major source of human exposure to fluoroquinolone resistance via food appears to be
poultry, whereas for cephalosporin resistance it is poultry, pork and beef that are important,
these food production systems require particular attention to prevent spread of such resistance
from these sources.
If a full risk assessment for a specific food-bacterium combination, in respect of AMR, should
be undertaken, methodologies currently available for the risk assessment of foods require to be
modified for uniform adaptation at both MS and EU level for the risk assessment of those
combinations (including foods originating from food animals, fish, fresh produce (e.g. lettuce
etc.) and water, as a vehicle for the transmission of AMR bacteria and related genes).
Further research on the role of commensals and of bacteria intentionally added as an aid to food
processing in the transmission of AMR via food to the human flora, aimed at identifying ways
in which such transmission from these agents can be prevented, is recommended.
The role of food, water and the environment in the spread of apparently epidemic plasmids
encoding multiple resistance is not clear, but deserves immediate attention.
Overall, control of all the routes by which AMR bacteria and their related genes can arise in the
human patient, of which food is but one such route, requires a response from all stakeholders to
acknowledge their responsibilities for preventing both the development and spread of AMR,
each in their own area of activity including medicine, veterinary medicine, primary food animal
production, food processing and food preparation, as well as in the regulation of food safety.
The EFSA Journal (2008) 765, 51-87
Foodborne Antimicrobial Resistance
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the development of antimicrobial resistance of importance for humans in Campylobacter and
Escherichia coli. Microbes and Infection, 1, 639-644.
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Foodborne Antimicrobial Resistance
APPENDICES
Table A:
Classes of antimicrobials, examples of substances used in human and veterinary medicine and examples of resistance genes.
Note: There is generally complete or partial cross resistance within each class or subclass unless otherwise indicated
Class
Examples of substances used in:
Human medicine
Veterinary medicine;
food production animals in EU
apramycin, gentamicin, streptomycin
neomycin, spectinomycin
Examples of
resistance genes
Comments
aac, aad (ant), aph,
armA, rpsL (strA)
rpsD, rpsE, strB
No general cross-resistance within class,
but some types of resistance will involve
cross-resistance between some
aminoglycosides
cfr confers cross-resistance to
amphenicols, lincosamindes,
pleuromutilins, streptogramins, linezolid
Cross resistance within subclasses but also,
depending on mechanism, between
subclasses
Aminoglycosides
amikacin, gentamicin, netilmicin, tobramycin
kanamycin, spectinomycin, streptomycin
Amphenicols
chloramphenicol, tiamphenicol
chloramphenicol, florfenicol,
tiamphenicol
cat, cfr, cml, flo
benzyl-penicillin, ampicillin, amoxicillin (with
clavulanic acid)
cloxacillin, dicloxacillin (meticillin)
benzyl-penicillin, ampicillin,
amoxicillin (with clavulanic acid)
cloxacillin, dicloxacillin
blaZ (bla-PC), bla-TEM.
bla-SHV, bla-OXA
bla-OXA, mecA
cephalexin, cefazolin, cephalotin
cefazolin, cephalexin
cefuroxime, loracarbef
-
bla-TEM. Bla-SHV,
bla-CTX, bla-CMY,
some bla-OXA
ceftazidime, ceftriaxone
ceftiofur
cefepime, cefpirome
cefepime, cefquinome
cefoxitin
ertapenem, imipenem, meropenem
-
Beta-lactam
antibiotics
Penicillins
Beta-lactamase
resistant penicillins
Cephalosporins, first
generation
Cephalosporins,
second generation
Cephalosporins,
third generation
Cephalosporins,
fourth generation
Cephamycins
Carbapenems
bla-CMY, bla-AAC
bla-IMP, bla-VIM, blaKPC some bla-OXA
The EFSA Journal (2008) 765, 72-87
Foodborne Antimicrobial Resistance
Class
Examples of substances used in:
Human medicine
Examples of
resistance genes
Comments
bcrABD
van (A-E)
Formerly used as feed additive in EU
Formerly avoparcin was used as feed
additive in EU
Used as coccidiostats
Cross-resistance also to macrolides and
streptogramin B for certain resistance
genotypes
Cyclic polypeptides
Glycopeptides
bacitracin
teicoplanin, vancomycin
Veterinary medicine;
food production animals in EU
(bacitracin)
(avoparcin)
Ionophores
Lincosamides
clindamycin, lincomycin
monensin, salinomycin
clindamycin, lincomycin
cfr, erm
Lipopeptides
Macrolides &
ketolides
daptomycin
erythromycin, spiramycin, azithromycin,
clarithromycin
spiramycin, tylosin, tulathromycin
erm, ere, mef, msr
Nitrofurans
Nitroimidazoles
furazolidone, nitrofurantoin
metronidazole, tinidazole
-
Orthosomycins
Oxazolidones
Pleuromutilins
Polymixins
Quinolones
avilamycin
tiamulin, valnemulin
colistin, polymixin B
danofloxacin, enrofloxacin,
Quinoxalines
linezolid
colistin, polymixin B
nalidixic acid, ciprofloxacin, norfloxacin,
moxifloxacin
-
carbadox, olaquindox
aac(6’)-Ib-cr, gyrA.
parC, qepA, qnr,
oqxAB
Streptogramins
pristinamycin, quinpristin/dalfopristin
(virginiamycin)
cfr, erm, vga , vgb
Sulphonamides &
trimethoprim
Tetracyclines
sulfadiazine, sulfamethoxazole, trimethoprim
sulfadiazine, sulfadoxine,
sulfamethoxazole, trimethoprim
chlortetracycline, doxycycline,
oxytetracycline
dfr, sul
chlortetracycline, doxycycline, oxytetracycline
emtA
cfr
cfr
Cross-resistance also to lincosamides and
streptograminB for certain resistance
genotypes
Used formerly as veterinary medicine
Dimetridazole and ronidazole used
formerly as veterinary medicine
Used formerly as feed additive
Incomplete cross-resistance. aac(6’)-Ib-cr
also confers resistance to kanamycin
Olaquindox used formerly as feed additive
in the EU
Formerly virginiamycin was used as feed
additive in EU
Cross-resistance between streptogramin B,
lincosamides and macrolides for certain
resistance genotypes
tet
The EFSA Journal (2008) 765, 73-87
Foodborne Antimicrobial Resistance
Class
Miscellaneous
Examples of substances used in:
Human medicine
Examples of
resistance genes
fosfomycin
fusidic acid
mupirocin
Veterinary medicine;
food production animals in EU
flavophospholipol (bambermycin)
fusidic acid
-
fosAB
fusB
mupA
rifampicin
(rifampicin)
rpoB
Comments
Used formerly as feed additive
Used in human medicine topically for
MRSA decontamination
Use in vet. med limited to foals
The EFSA Journal (2008) 765, 74-87
Foodborne Antimicrobial Resistance
Ciprofloxacin/Enrofloxacin
Nalidixic acid
Gentamicin
Neomycin-/kanamycin
Streptomycin
beef
40
2
-
2
2*
5
0
0
12
-
12
2
Remost 2004
2005
beef
238
13
2
4
1
2
-
-
12
19
16
11
EFSA 2006
Denmark
2004
beef
196
8
0
1
0*
0
0
2
9
7
9
4
DANMAP 2005
The Netherlands
2004
beef
34
12
3
3
9*
3
0
0
-
15
12
12
MARAN 2005
Norway
2005
beef
90
3
0
0
0
0
0
0
10
3
2
3
EFSA 2006
Austria
2003
poultry
34
26
-
0
30*
32
4
0
35
-
38
18
Remost 2004
Belgium
2005
broiler
148
37
3
7
3
28
-
-
24
37
39
25
EFSA 2006
Denmark
2004
broiler
216
15
0
<1
0*
6
0
0
1
15
9
3
DANMAP 2004
The Netherlands
2004
poultry
115
54
11
8
30*
33
4
12
-
50
47
43
MARAN 2005
Austria
2003
pork
56
16
-
12
4*
4
0
2
54
-
55
12
Remost 2004
Belgium
2005
pork
86
10
-
7
1
2
-
-
19
15
21
15
EFSA 2006
Denmark
2004
pork
178
15
0
2
0*
2
2
3
13
18
26
10
DANMAP 2004
The Netherlands
2004
pork, organic
155
16
1
6
0*
0
4
38
-
27
38
17
MARAN 2005
Food type
Number of
isolates
Trimethoprim
Chloramphenicol
2003
Year
Tetracycline
3rd gen cephalosporin
Austria
Belgium
Country
Sulphonamides
Ampicillin
Table B. Occurrence of resistance to antimicrobials in Escherichia coli from food products (percent resistant isolates)a (Sources: The Community Summary Report on Trends and Sources of
Zoonoses, Zoonotic Agents, Antimicrobial Resistance and Foodborne Outbreaks in the European Union in 2005 and national reports)
Reported resistance (%)
Data source
Germany
2005
mixed meat
50
2
0
0
0
-
0
0
10
14
12
4
EFSA 2006
Portugal
2005
cheese
33
30
0
3
6
-
36
42
91
-
58
-
EFSA 2006
CIPARS 2003
Non-EU countries
Canada QC
2003
broiler
112
50
33
18
0*
1
18
11
48
43
57
-
Canada; ON
2003
broiler
136
35
18
5
2*
2
7
9
32
24
51
-
CIPARS 2003
Canada QC
2003
pork
61
20
2
10
0*
0
2
3
28
31
48
-
CIPARS 2003
Canada ON
2003
pork
91
20
2
8
0*
0
1
6
17
30
55
-
CIPARS 2003
Canada QC**
2003
beef
84
7
0
1
1*
1
1
2
2
7
19
-
CIPARS 2003
Canada ON**
2003
beef
100
8
2
2
0*
0
0
2
6
14
23
-
CIPARS 2003
* cut-off of >0.06 i.e. the same as for DANMAP has been used to define resistance for the compilation of this table; ** ON = Ontario, QC = Quebec
The EFSA Journal (2008) 765, 75-87
Foodborne Antimicrobial Resistance
References for Table B:
CIPARS (Canadian Integrated Program for Antimicrobial Resistance Surveillance), 2003. Available at; www.phac-aspc.gc.ca/ciparspicra/pdf/cipars-picra-2003_e.pdf. Accessed 12 February 2008.
DANMAP, 2005. Use of antimicrobial agents and occurrence of resistance in bacteria from food animals, foods and humans in Denmark. ISSN
1600-2032 www.dfvf.dk).
EFSA, 2006. The Community Summary Report on Trends and Sources of Zoonoses, Zoonotic Agents, Antimicrobial Resistance and Foodborne
Outbreaks in the European Union in 2005. The EFSA Journal (2006), 94
MARAN, 2005. Monitoring of antimicrobial resistance
http://library.wur.nl/way/bestanden/clc/1865472_2005.pdf
and
antibiotic
usage
in
the
Netherlands
in
2004.
REMOST, 2004. Resistensmonitoring Steiermark 2003 - Eine flächendeckende Erhebung zum Resistenzverhalten von ausgewählten
Zoonoseerregen, Indikatorbakterien und euterpathogenen Keimen in der steirischen Nutztierpopulation. Projektbericht, Fachabteilung 8C Veterinärwesen amt der steiermärkischen Landeregierung.
The EFSA Journal (2008) 765, 76-87
Foodborne Antimicrobial Resistance
Table C:
Qualitative risk assessment for fluoroquinolone-resistant Campylobacter jejuni in the UK: example of use of template.
Please note - Data used is that which was readily available to working group or from informal expert opinion.
THIS IS NOT A FORMAL RISK ASSESSMENT.
Food category
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
food
1. Milk and
dairy products
(cows, goats
sheep, buffalo,
horse)
1.1 Milk
A. Fresh or raw
19/1097 (1.7%) unpasteurised cows’ milk
samples positive. (de Louvois &
Rampling, 1998)
Data from abattoir study used as an indicator of
probability of antimicrobial resistance at retail (Teale,
2002).18 0/99 C. jejuni cattle isolates were resistant
to nalidixic acid or ciprofloxacin. 0/65 C. jejuni
sheep isolates were resistant to nalidixic acid or
ciprofloxacin.
Assumption.
Scotland.
Prohibited from sale in
0/100 of unpasteurised goats’ milk
samples positive (Little & de Louvois,
1999)
1.2 Dairy products
0/26 of unpasteurised ewe’s milk samples
positive (Little & de Louvois, 1999).
Also - referred to data for bovine/sheep meat
B. Minimally
processed
Assumption.
Assumption.
Lower probability than for raw milk.
Same as raw milk.
C. Processed
Pasteurisation very effective at killing
Campylobacter. However outbreaks have
occurred where pasteurisation has failed
or from bird-pecked milk.
Assumption.
Assumption.
Assumption.
Same as raw milk.
Same as raw milk.
A. Fresh or raw
C. Processed
1.3 Cheese
A. Fresh or raw
Same as raw milk.
purchased
and
Assumption.
99.3% of participants in Irish survey
consumed milk (Harrington et al., 2001).
Assumed that majority is pasteurised.
Assumption. Raw cows' cream prohibited
from sale of in Scotland.
Assumption.
Assumption.
Same as processed milk.
Same as raw milk.
74.6% of participants in Irish survey
consumed dairy products (Harrington et al.,
2001). Assumed that majority is purchased
processed / pasteurised.
Assumption. Risk for cheese made from
unpasteurised milk is assumed to be very
low. This takes into account the risk for
unpasteurised milk and also maturation
time.
Assumption.
Assumption.
Same as raw milk.
17
UK data (MAFF 2000) readily available to the working group gave % of all household purchasing each type of food in survey week, which was unsuitable for the risk assessment template;
therefore Irish consumption data were used.
18
Breakpoint of 16 mg/ml for nalidixic acid; 1 mg/ml for ciprofloxacin
The EFSA Journal (2008) 765, 77-87
Foodborne Antimicrobial Resistance
Food category
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
B. Minimally
processed
(smoked)
Assumption.
Assumption.
Assumption.
C. Processed
Assumption.
A. Fresh or raw
purchased
and
Same as raw milk.
Assumption.
Same as raw milk.
2. Egg and egg
products
food
0/226 eggs produced from hens faecally
shedding C. jejuni were positive; 2 of the
shell surfaces were C. jejuni positive
(Doyle, 1984).
78.0% of participants in Irish survey
consumed cheese (Harrington et al., 2001).
Assumed that majority is purchased
processed / pasteurised.
Assumption. Same fresh or raw broiler meat.
However, use of quinolones may significantly differ
between layers and broilers - high level of uncertainty
92.2% of participants in Irish survey
consumed egg & egg products (Harrington et
al., 2001). Assumed that majority purchased
as raw.
2/187 (1.1%) eggs produced from hens
faecally shedding C. jejuni were positive
due to penetration of the egg shell. 0/142
eggs derived from birds of unknown
status were C. jejuni positive (Shanker et
al., 1986)
3. Red meats
3.1 Bovine
B. Minimally
processed (as in
desserts)
Assumption. Lower probability than for
fresh or raw eggs.
Assumption. Same as fresh or raw eggs.
Assumption.
C. Processed
Assumption. Lower probability than for
fresh or raw eggs.
Assumption. Same as fresh or raw eggs.
Assumption.
A. Fresh or raw
71/1514 (4.7%) of meat cuts and 6/49
(12.2%) offal portions were positive for
Campylobacter. 43/49 (87.7%) isolates
were C. jejuni (Little et al., 2008)
13.9% of C. jejuni resistant to nalidixic acid; 11.6%
resistant to ciprofloxacin (43 isolates tested) (Little et
al., 2008)19
87.8% of participants in Irish survey
consumed bovine meat and products
(Harrington et al. 2001). Assumed that
majority is purchased as raw and as meat cuts
(i.e. not offal).
47/96 (49%) of ox liver samples were
positive for C. jejuni. (Kramer et al,
2000)
15.1% of 53 C. jejuni isolates isolated from ox liver
were resistant to nalidixic acid; 3.8% were resistant
to ciprofloxacin20. (Kramer et al., 2000)
19
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
20
Kramer et al. 2000 used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin.
The EFSA Journal (2008) 765, 78-87
Foodborne Antimicrobial Resistance
Food category
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
food
purchased
B. Minimally
processed
(cured and/or
smoked)
Assumption.
Assumption. Same as fresh or raw bovine meat.
Assumption
C. Processed
0/3085 ready-to-eat burgers (of which
90% were beef) purchased from burger
outlets were positive for Campylobacter
(Little et al., 2001).
Assumption. Same as fresh or raw bovine meat.
Assumption.
Significant
purchased as processed.
27.8% of C. jejuni resistant to nalidixic acid; 19.4%
resistant to ciprofloxacin (36 isolates tested) (Little et
al., 2008)21
93.7% of participants in Irish survey
consumed pig meat and products (Harrington
et al. 2001). Assumed that significant
proportion is purchased as raw (includes
sausages) and not as offal.
proportion
and
is
1/546 (0.18%) ready to eat beef (cold)
positive for Campylobacter (Elson et al.,
2004)
0/371 VP-MAP ready to eat beef positive
for Campylobacter (Sagoo et al., 2007)
3.2 Pig
A. Fresh or raw
66/1309 (5%) of meat cuts and 24/131
(18.3%) offal portions were positive for
Campylobacter. 36/68 (52.9%) isolates
were C. jejuni (Little et al., 2008)
34/99 (34.3%) of pigs liver samples were
positive for C. jejuni. (Kramer et al.,
2000)
B. Minimally
processed
(cured and/or
smoked)
Assumption. Lower probability than for
fresh or raw pig meat.
33.3% of 36 C. jejuni isolates isolated from pigs liver
were resistant to nalidixic acid; 5.6% were resistant
to ciprofloxacin22. (Kramer et al., 2000)
Assumption. Same as fresh or raw pig meat.
21
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
22
Kramer et al. 2000 used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin.
93.7% of participants in Irish survey
consumed pig meat and products (Harrington
et al. 2001). Assumed that significant
proportion is purchased as minimally
processed (includes bacon).
The EFSA Journal (2008) 765, 79-87
Foodborne Antimicrobial Resistance
Food category
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
C. Processed
0/1423 ready to eat ham (cold) positive
for Campylobacter. 0/243 ready to eat
pork (cold) positive for Campylobacter.
(Elson et al., 2004)
Assumption. Same as fresh or raw pig meat.
93.7% of participants in Irish survey
consumed pig meat and products (Harrington
et al. 2001). Assumed that significant
proportion is purchased as processed
(includes ham).
12.5% of C. jejuni resistant to nalidixic acid; 10.9%
resistant to ciprofloxacin (64 isolates tested) (Little et
al. , 2008)23
34.5% of participants in Irish survey
consumed sheep meat and products
(Harrington et al. 2001). Assumed that
majority is purchased as raw and not as offal.
0/1351 VP-MAP ready to eat ham
positive for Campylobacter. 0/206 VPMAP ready to eat pork positive for
Campylobacter (Sagoo et al., 2007)
3.3 Sheep
A. Fresh or raw
55/744 (7.4%) of meat cuts and 59/161
(36.6%) offal portions were positive for
Campylobacter. 64/90 (71.1%) isolates
were C. jejuni (Little et al., submitted)
72/96 (75%) of lambs liver were positive
for C. jejuni. (Kramer et al., 2000).
7% of 100 C. jejuni isolates isolated from lambs liver
were resistant to nalidixic acid; 4% were resistant to
ciprofloxacin24. (Kramer et al. 2000).
food
purchased
and
B. Minimally
processed
(cured and/or
smoked)
Assumption. Lower probability than for
fresh or raw sheep meat.
Assumption. Same as fresh or raw sheep meat.
Assumption.
C. Processed
0/19 ready to eat lamb (cold) positive for
Campylobacter (Elson et al., 2004)
Assumption. Same as fresh or raw sheep meat.
Assumption.
GAME & OTHER MEATS: 0% of C. jejuni resistant
to nalidixic acid; 0% resistant to ciprofloxacin (3
isolates tested) (Little et al., 2008)26
4.1% of participants in Irish survey
consumed ‘other’ red meat and products
(Harrington et al. 2001). Assumed that
majority is purchased as raw and as meat
cuts.
Note - low sample size.
Assumption. Lower probability than for
fresh or raw sheep meat.
3.4 Other
A. Fresh or raw
GAME & OTHER MEATS25: 5/47
(10.6%) of meat cuts; 0/1 (0%) offal
portions and 0/3 (0%) whole animals
were positive for Campylobacter. 3/4
(75%) were C. jejuni (Little et al., 2008)
Note - low sample size.
Note - low sample size.
Assumption.
23
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
24
Kramer et al. 2000 used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin.
25
hare, rabbit, venison, goat, mutton
26
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
The EFSA Journal (2008) 765, 80-87
Foodborne Antimicrobial Resistance
Food category
4. Poultry meats
Food sub-category
4.1 Broiler
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
B. Minimally
processed
(cured and/or
smoked)
Assumption. Lower probability than for
fresh or raw ‘other’ meat.
Assumption. Same as fresh or raw ‘other’ red meat.
Assumption.
C. Processed
Assumption. Lower probability than for
fresh or raw ‘other’ meat.
Assumption. Same as fresh or raw ‘other’ red meat.
Assumption
A. Fresh or raw
In large UK study, 50% of chickens
sampled (5394) were positive for
Campylobacter spp. [56% fresh chicken;
31% frozen chicken]. Of 1636 isolates
tested, 74% were C. jejuni. (Food
Standards Agency, 2003).
In large UK study, resistance to ciprofloxacin was
detected in 13% of C. jejuni isolates. (Food
Standards Agency, 2003).
84.3 % of participants in Irish survey
consumed broiler meat and products
(Harrington et al., 2001). Assumed that
majority is purchased as raw.
187/301 (62.1%) whole birds and
896/1477 (60.7%) portions were positive
for Campylobacter. 163/239 (68.2%)
were C. jejuni (Little et al., submitted).
187/595 (31.4%)and 12/595 (2.0%) Campylobacter
spp. isolates (from raw whole chickens) resistant to
nalidixic acid and ciprofloxacin, respectively28
(Anon., 2005).
In Northern Ireland study 141/412 (34%)
of local whole chickens were C. jejuni
positive. From imported (frozen) chicken
breasts 33/150 (22%) were C. jejuni
positive. (Wilson, 2003).
In Northern Ireland study, 9/141 (6.4%) of isolates
from local whole chickens were resistant to nalidixic
acid and 12/141 (8.5%) resistant to ciprofloxacin.
From imported (frozen) chicken breasts, 6/33
(18.1%) were resistant to nalidixic acid and 6/33
(18.1%) resistant to ciprofloxacin. 29 (Wilson, 2003).
156/198 (77.3%) of chilled chicken breast
or thigh portions were positive for C.
jejuni. (Kramer et al., 2000).
B. Minimally
processed
(cured and/or
smoked)
Assumption.
11% of C. jejuni resistant to nalidixic acid; 9.4%
resistant to ciprofloxacin (64 isolates tested) (Little et
al., submitted)27
food
purchased
15% of 194 C. jejuni isolates were resistant to
nalidixic
acid;
10.8%
were
resistant
to
ciprofloxacin30. (Kramer et al., 2000).
Assumption. Same as fresh or raw broiler meat.
27
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
28
Anon. 2005 used the HPA breakpoints, i.e 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
29
Wilson, 2003 used the following concentrations of antimicrobials in the discs suscepbility testing: 30µg for nalidixic acid; 1µg for ciprofloxacin.
30
Kramer et al. 2000 used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin.
Assumption
The EFSA Journal (2008) 765, 81-87
and
Foodborne Antimicrobial Resistance
Food category
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
food
purchased
and
C. Processed
0/121 ready to eat chicken (cold) positive
for Campylobacter (Elson et al., 2004)
Assumption. Same as fresh or raw broiler meat.
Assumption
16.7% of C. jejuni resistant to nalidixic acid; 16.7%
resistant to ciprofloxacin (6 isolates tested) (Little et
al., submitted)31
24.1 % of participants in Irish survey
consumed turkey meat and products
(Harrington et al., 2001). Assumed that a
significant proportion is purchased as raw.
0/495 VP-MAP ready to eat chicken
positive for Campylobacter (Sagoo et al.,
2007)
0/449 chicken sandwich samples were
positive for Campylobacter (Little et al.,
2002).
4.2 Turkey
A. Fresh or raw
1/2 (50%) of whole birds and 71/212
(33.5%) portions were positive for
Campylobacter. 7/15 (46.7%) were C.
jejuni. (Little et al., submitted)
Note - low sample size.
B. Minimally
processed
(cured and/or
smoked)
Assumption. Lower probability than fresh
or raw turkey meat
Assumption. Same as fresh or raw turkey meat.
24.1 % of participants in Irish survey
consumed turkey meat and products
(Harrington et al., 2001). Assumed that a
lesser proportion is purchased as minimally
processed.
C. Processed
0/411 ready to eat turkey (cold) positive
for Campylobacter (Elson et al., 2004)
Assumption. Same as fresh or raw turkey meat.
24.1 % of participants in Irish survey
consumed turkey meat and products
(Harrington et al., 2001). Assumed that a
significant proportion is purchased as
processed.
DUCK: 2/7 (28.6%) of whole birds and
37/70 (52.9%) portions were positive for
Campylobacter. 8/19 (42.1%) isolates
were C. jejuni. (Little et al., submitted)
DUCK. 0% of C. jejuni resistant to nalidixic acid; 0%
resistant to ciprofloxacin (9 isolates tested) (Little et
al., submitted)
2.3% of participants in Irish survey consumed
other poultry meat and products (Harrington
et al. 2001). Assumed that majority is
purchased as raw.
OTHER32: 11/23 (47.8%) of whole birds
and 1/12 (8.3%) portions were positive
for Campylobacter. 2/4 (50.0%) were C.
jejuni. (Little et al., submitted)
OTHER: 0% of C. jejuni resistant to nalidixic acid;
0% resistant to ciprofloxacin (3 isolates tested) (Little
et al., submitted)33
1/523 VP-MAP ready to eat turkey
positive for Campylobacter (Sagoo et al.,
2007)
4.3 Other
A. Fresh or raw
Note - low sample size
Note - low sample sizes.
Assumption. Same as fresh chicken & turkey.
31
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
32
grouse, guinea fowl, ostrich, partridge, pheasant, poussin, quail, wood pigeon
The EFSA Journal (2008) 765, 82-87
Foodborne Antimicrobial Resistance
Food category
5. Aquaculture
and marine
Food sub-category
5.1 Fish
5.2 Crustaceans,
shellfish, molluscs
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
B. Minimally
processed
(cured and/or
smoked)
Assumption.
Assumption. Same as fresh or raw ‘other’ poultry
meat.
Assumption
C. Processed
Assumption.
Assumption. Same as fresh or raw ‘other’ poultry
meat.
Assumption
A. Fresh or raw
Assumption
Assumption.
65.1% of participants in Irish survey
consumed fish and fish products (Harrington
et al. 2001). Assumed that significant
proportion is purchased as raw.
B. Minimally
processed
(pickled and/or
smoked)
Assumption
Assumption.
Assumption
C. Processed
Assumption
Assumption.
65.1% of participants in Irish survey
consumed fish and fish products (Harrington
et al. 2001). Assumed that significant
proportion is purchased as processed.
A. Fresh or raw
In Irish study, 3/117 (2.5%) of seafood
sampled (oysters and mussels) were C.
jejuni positive (Whyte et al., 2004).
Assumption.
8.8% of participants in Irish survey consumed
crustaceans,
shellfish
and
molluscs
(Harrington et al., 2001). Assumed that small
proportion is purchased as processed.
Assumption.
Assumption.
47% of 331 mixed bivalves (cockles,
mussels, scallops) shortly after harvesting
were positive for Campylobacter spp.
Only 2% of these were C. jejuni. (Wilson
& Moore, 1996).
B. Minimally
processed
33
Assumption
food
purchased
Little et al., (submitted) used a breakpoint of 16mg/litre for nalidixic acid and 1 mg/litre for ciprofloxacin
The EFSA Journal (2008) 765, 83-87
and
Foodborne Antimicrobial Resistance
Food category
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
C. Processed
3/49 (6%) of depurated oysters were
positive for Campylobacter spp. None
were C. jejuni. (Wilson & Moore, 1996).
Assumption.
8.8% of participants in Irish survey consumed
crustaceans,
shellfish
and
molluscs
(Harrington et al., 2001). Assumed that
majority is purchased as processed.
A. Fresh or raw
0/2870 open ready to eat salad samples
positive for Campylobacter (Sagoo, et al.,
2003a)
Assumption. Animal/human wastes spread onto land
99.9% of participants in Irish survey
consumed vegetables & juices and products
(Harrington et al., 2001). Assumed that
majority purchased as raw.
Note - low sample size for C. jejuni.
6. Vegetables,
cereals, fruits
6.1. Vegetables and
juices
0/3827 ready to eat salad vegetable
samples positive for Campylobacter
(Sagoo et al., 2003b)
food
purchased
and
0/151 unprepared non-UK whole lettuce
positive for Campylobacter (Little et al.,
1999)
0/2883 ready-to-eat organic vegetables
positive for Campylobacter (Sagoo et al.,
2001)
6.2 Cereal products
B. Minimally
processed
(pickled
vegetables)
Assumption. Lower probability than for
fresh or raw vegetables.
Assumption. Same as fresh/raw
Assumption.
C. Processed
Assumption. Lower probability than for
minimally processed vegetables.
Assumption. Same as fresh/raw
99.9% of participants in Irish survey
consumed vegetables & juices and products
(Harrington et al., 2001). Assumed that
significant proportion is purchased as
processed.
A. Fresh or raw
Assumption.
Assumption. Animal/human wastes spread onto land
100% of participants in Irish survey
consumed cereal products (Harrington et al.,
2001). Assumed that large proportion is
purchased as fresh/raw.
B. Minimally
processed
Assumption. Lower probability than for
fresh/raw cereals
Assumption. Same as fresh/raw
Assumption
C. Processed
Assumption. Lower probability than for
fresh/raw cereals
Assumption. Same as fresh/raw
100% of participants in Irish survey
consumed cereal products (Harrington et al.,
2001). Assumed that majority are purchased
as processed.
The EFSA Journal (2008) 765, 84-87
Foodborne Antimicrobial Resistance
Food category
7. Herbs and
spices
Food sub-category
Processing
factors
Probability of bacteria being present in
food at retail
Probability that bacteria present in food at retail is
resistant to antimicrobial class of interest
Probability
consumed17
food
purchased
and
6.3 Fruit, berries
and juices
A. Fresh or raw
0/143 strawberries were positive for
Campylobacter spp.; 0/162 melons were
positive for Campylobacter spp.
(Williamson et al., 2003)
Assumption.
91.4% of participants in Irish survey
consumed fruits, berries, juices and products
(Harrington et al., 2001). Assumed that
majority are purchased raw.
B. Minimally
processed
Assumption
Assumption.
Assumption
C. Processed
Assumption
Assumption.
Assumption
A. Fresh or raw
Assumption
Assumption. Animal/human wastes spread onto land
58.1% of participants in Irish survey consumed
herbs and spices (Harrington et al., 2001).
Assumed that lesser proportion are purchased as
fresh herbs/spices.
B. Minimally
processed
Assumption
Assumption. Same as fresh/raw herbs and spices
Assumption
C. Processed
Assumption
Assumption. Same as fresh/raw herbs and spices
58.1% of participants in Irish survey
consumed herbs and spices (Harrington et al.,
2001). Assumed that majority are purchased
as processed (i.e. dried).
A. Not
chlorinated
Assumption
Assumption.
Private water supplies may be
contaminated by run-off from nearby land
Assumption
B. Chlorinated
Assumption
Assumption. Same as unchlorinated water.
94.2% of participants in Irish survey
consumed tap water (Harrington et al., 2001).
Assumed that majority is chlorinated.
8. Mixed or
buffet meals*
9. Other foods*
10. Tap water,
including wellwater
* As assessed in respect of the food component subjected to the least amount of heat treatment or exposure to comparable treatment, e.g. raw meat, raw vegetable, smoked fish.
The EFSA Journal (2008) 765, 85-87
Foodborne Antimicrobial Resistance
References for Table C:
Anon., 2005. United Kingdom: Trends and Sources of Zoonoses and zoonotic agents in
humans, foodstuffs, animals and feeding stuffs in 2005.
www.defra.gov.uk/animalh/diseases/zoonoses/zoonoses_reports/report2005uk.pdf
de Louvois, J., and Rampling, A., 1998. One fifth of samples of unpasteurised milk are
contaminated with bacteria. B.M.J., 316, 625
Doyle, M.P., 1984. Association of Campylobacter jejuni with Laying Hens and Eggs. Appl.
Environ. Microbiol. 47, 533-536.
Elson, R., Burgess, F., Little, C.L. and Mitchell, R.T. on behalf of the Local Authorities Coordinators of Regulatory Services and the Health Protection Agency, 2004. J. Appl. Microbiol.,
96, 499 - 509.
Food Standards Agency, 2003. Food Standards Agency - UK-wide survey of Salmonella and
Campylobacter contamination of fresh and frozen chicken on retail sale. Available at:
www.food.gov.uk/multimedia/webpage/111802
Harrington, K.E., Robson, P.J., Kiely, M., Livingstone, M.B.E., Lambe, J. and Gibney, M.J.,
2001. The North/South Ireland food consumption survey: survey design and methodology.
Public Health Nutrition 4(5A), 1037-1042.
Kramer, J.M., Frost, J.A., Bolto, F. and Wareing, D.R.A., 2000. Campylobacter contamination
of raw meat and poultry at retail sale: Identification of multiple types and comparison with
isolates from human infection. J. Food Protect., 63, 1654-1659.
Little, C.L., Barnes, J. and Mitchell, R.T., on behalf of the Food Standards Agency (FSA) and
the Public Health Laboratory Service (PHLS), 2001. Micrbiologilcal examination of ready-toeat burgers sampled anonymously at the point of sale in the United Kingdom. Communicable
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